Poster Note 64374

Evaluation of Bench-top Quadrupole Orbitrap Ultra High Resolution MS for Use in Clinical Research in Rapid Quantitative Analysis of Vitamin D in Human Plasma

Mindy Gao and Marta Kozak Thermo Fisher Scientific, San Jose, CA, USA

2 Evaluation of Bench-top Quadrupole Orbitrap Ultra High Resolution MS for Use in Clinical Research in Rapid Quantitative Analysis of Vitamin D in Human Plasma

TABLE 4. Intra-assay Precision and Accuracy *

021715_APCI_4xP_D1_Cal_7 #752 RT: 1.13 AV: 1 NL: 5.82E6F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00]

50 100 150 200 250 300 350 400m/z

0

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383.3298

365.3195

257.2257

121.1012245.225695.0857 135.1167 159.1164 191.1792 269.2241 309.256669.0704

225.1631

327.2668

Conclusion Method meets clinical research requirements for analysis of Vitamin D

25-hydroxy metabolites in plasma samples.

The calibration range used in method evaluation experiments was 1 to 100 ng/mL, but for improved method robustness, recommended concentration range is 4-100 ng/mL.

Deuterated analog of 25OHD2 is recommended to correct for limited matrix effects we observed during method evaluation.

Purpose To evaluate a rapid quantitative analysis of Vitamin D in human plasma samples using a bench-top quadrupole orbitrap high resolution mass spectrometer for use in clinical research.

Introduction Clinical researchers commonly use a triple quadrupole mass spectrometer for analysis of 25-hydroxyvitamin D2 (25OHD2) and 25-hydroxyvitamin D3 (25OHD3) in plasma. We evaluated the Thermo Scientific™ Q Exactive™

Focus mass spectrometer equipped with Thermo Scientific™ Orbitrap™ technology using a fast, cost-efficient method that collected high resolution MS/MS spectra for improved method specificity. Protein precipitated plasma samples were analyzed with 3 min LC method, and high resolution MS/MS spectra were collected for each analyte. The most abundant fragment, besides water-loss, in each MS2 spectrum was selected for quantitative analysis (Table 3, Figure 1). The linearity range was 4-100 ng/mL (Figure 3, Figure 4); precision and accuracy were within 15%; matrix effects and interferences were not observed.

Instruments LC system

Pump: Thermo Scientific TM Dionex TM Ultimate TM 3000 Autosampler: Thermo Scientific TM OAS-3X00TXRS

Q Exactive Focus orbitrap mass spectrometer

Methods Calibrators

25-hydroxyvitamin D2 (25OHD2), 25-hydroxyvitamin D3 (25OHD3) were purchased from Cerillant Corporation. Since analyte free matrix was not available, calibration standards were prepared in ethanol. NIST controls and spiked plasma recovery data were used to prove calibration curve accuracy.

Sample Preparation

1.100 µL of plasma sample + 300 uL of acetonitrile containing internal standard (25 ng/mL d6-25-hydroxyvitamin D3 ). 2.Vortex, centrifuge 3.Inject 50 µL into LC-MS system.

LC method

Mobile phase A: 0.1% formic acid in water Mobile phase B: 0.1% formic acid in methanol Column: Thermo Scientific TM Hypersil GOLDM aQ 5µ 50x2.1mm

TABLE 1. HPLC Gradient Method

Mass Spectrometry Method

APCI ionization source

Data acquisition method: parallel reaction monitoring (PRM) experiment collecting MS2 spectra for each analyte.

Resolution: 17.5K

Data Analysis

Thermo Scientific™ TraceFinder 3.2 software was used for all data processing and analysis.

Method Performance Evaluation QC samples were prepared by spiking previously analyzed donor plasma to concentrations specified in Table 2 and Figure 2.

TABLE 2. QC Samples Concentrations

Results FIGURE 1. 25OHD2, 25OHD3 MS/MS Spectrum

FIGURE 2. Chromatogram of QC Plasma Samples

QC1 QC2 QC3

25OHD2

25OHD3

6-25OHD3

(IS)

FIGURE 3. Calibration Curves with Lowest Calibration Standard Peaks

25OHD2

4.0 ng/mL

25OHD3

4.0 ng/mL

d6-25OHD3

(IS), 25 ng/mL

©2015 Thermo Fisher Scientific. All Rights Reserved.

All other trademarks are the property of Thermo Fisher Scientific and its subsidiaries.

This information is not intended to encourage use of these products in any manners that might infringe the intellectual property rights of others.

Evaluation of Bench-top Quadrupole Orbitrap Ultra High Resolution MS for Use in Clinical Research in Rapid Quantitative Analysis of Vitamin D in Human Plasma Mindy Gao, Marta Kozak Thermo Fisher Scientific, San Jose, CA, USA

For research use only. Not for use in diagnostic procedures.

Time (min) Flow rate (mL/min) %A (mobile phase) 0 0.70 20 0.2 0.70 20 0.3 0.70 5 1.5 0.70 5 1.6 0.70 20 2.0 0.70 20

021715_APCI_4xP_D1_Cal_7 #787 RT: 1.17 AV: 1 NL: 3.64E6F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00]

50 100 150 200 250 300 350 400m/z

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395.3300

377.3193

269.1893

83.0860229.1583119.0856

209.1322251.1792135.1168 159.1163 185.1320 307.2419

279.2106

335.2729

Water lost fragment

Quantifier

25OHD2

Quantifier

Water lost fragment

25OHD3

RT: 0.00 - 2.00 SM: 5B

0.0 0.5 1.0 1.5 2.0Time (min)

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1001.17

1.13

1.13

NL: 7.56E4m/z= 269.1848-269.1948 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_PlasmaL_5

NL: 1.99E5m/z= 257.2214-257.2314 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_PlasmaL_5

NL: 2.07E6m/z= 263.2588-263.2688 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_PlasmaL_5

RT: 0.00 - 2.00 SM: 5B

0.0 0.5 1.0 1.5 2.0Time (min)

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1001.18

1.12

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NL: 1.54E5m/z= 269.1848-269.1948 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_PlasmaM_2

NL: 3.63E5m/z= 257.2214-257.2314 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_PlasmaM_2

NL: 2.65E6m/z= 263.2588-263.2688 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_PlasmaM_2

RT: 0.00 - 2.00 SM: 5B

0.0 0.5 1.0 1.5 2.0Time (min)

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1001.17

1.12

1.12

NL: 2.38E5m/z= 269.1848-269.1948 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_PlasmaH_2

NL: 5.64E5m/z= 257.2214-257.2314 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_PlasmaH_2

NL: 2.62E6m/z= 263.2588-263.2688 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_PlasmaH_2

10.0 ng/mL 30.0 ng/mL 20.0 ng/mL

Collision energy (20 eV) was optimized to maximize response of quantifying fragment ion (m/z=269.1893)

Collision energy (15 eV) was optimized to maximize response of quantifying fragment ion (m/z=257.2257)

25.1 ng/mL 39.9 ng/mL 60.8 ng/mL

4 ng/mL 4 ng/mL

Calculated Amt %Diff 3.98 -0.450 9.97 -0.280 26.1 4.50 50.1 0.120 96.1 -3.88

Calculated Amt %Diff 3.96 -1.10 10.2 1.95 26.3 5.08 46.7 -6.58 101 0.640

Analyte QC1 QC2 QC3 %RSD

25-Hydroxyvitamin D2 6.30 - 12.7 5.33 - 13.0 2.77 - 5.30 25-Hydroxyvitamin D3 3.21 - 7.64 2.64 - 5.89 3.70 - 4.70

%Recovery 25-Hydroxyvitamin D2 87.0 - 100 99.9 - 109 102 - 106 25-Hydroxyvitamin D3 82.9 - 83.5 94.5 - 96.3 91.1 - 101

* 5 replicates of QC samples containing 25OHD2 and 25OHD3 were proceed and analyzed in 3 batches

Analyte QC1 QC2 QC3 %RSD

25-Hydroxyvitamin D2 10.5 9.01 4.51 25-Hydroxyvitamin D3 5.56 3.93 6.1

%Recovery 25-Hydroxyvitamin D2 93.2 105 104 25-Hydroxyvitamin D3 82.9 95.1 97.3

* 5 replicates of QC samples containing 25OHD2 and 25OHD3 were proceed and analyzed in 3 batches

Compound Precursor (m/z)

Quantitation Fragment (m/z)

Collision Energy (V) Polarity

25OHD2 395.3308 269.1898 20 Positive 25OHD3 383.3308 257.2264 15 Positive D6-25OHD3 (IS) 389.3685 263.2638 20 Positive

Analyte Cal-4 Cal-10 Cal-25 Cal-50 Cal-100 %RSD

25OHD2 1.60 2.52 4.27 1.65 2.71 25OHD3 4.72 1.37 4.77 2.01 3.86

%Recovery 25OHD2 99.7 101 96.8 105 96.9 25OHD3 100 101 97.0 98.8 103

* 5 replicate injections of each calibration standard containing 25OHD2 and 25OHD3 were performed to demonstrate the system reproducibility

Analyte Plasma-1 Plasma-2 Plasma-3 Plasma-4 Plasma-5 %RSD

25OHD2 3.65 5.36 9.17 5.90 10.6 25OHD3 2.70 3.48 1.09 4.31 6.99

%Recovery 25OHD2 77.2** 91.7 79.9** 86.5 85.3 25OHD3 112 104 106 109 111

* 15 ng/mL of each analyte was spiked in 5 different plasma samples in 5 replicates

** 25OHD2 % recovery will be increased when deuterated analog will be used as internal standard.

FIGURE 4. Chromatogram of Lowest Calibration Standard

RT: 0.80 - 1.50 SM: 5B

0.8 0.9 1.0 1.1 1.2 1.3 1.4 1.5Time (min)

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NL: 2.66E4m/z= 269.1885-269.1911 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_Cal_3

NL: 4.23E4m/z= 257.2251-257.2277 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_Cal_3

NL: 2.24E6m/z= 263.2625-263.2651 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_Cal_3

RT: 0.80 - 1.50 SM: 5B

0.8 0.9 1.0 1.1 1.2 1.3 1.4 1.5Time (min)

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NL: 2.66E4m/z= 269.1885-269.1911 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_Cal_3

NL: 4.23E4m/z= 257.2251-257.2277 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_Cal_3

NL: 2.24E6m/z= 263.2625-263.2651 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_Cal_3

Chromatogram reconstructed with mass accuracy of 5 ppm

System reproducibility was evaluated by analyzing 5 replicates of each calibration standard (Table 6). TABLE 3. PRM transitions of targets and internal standards

Method accuracy was evaluated by obtaining %recovery for NIST controls.

Method precision was evaluated by analyzing 5 replicates of each QC sample in 3 different days (Table 4, Table 5).

Matrix effects were evaluated by spiking previously analyzed plasma from 5 different donors with 25OHD3 and 25OHD2 concentrations of 15 ng/mL and calculating % RSD and % recovery from 5 replicate analysis (Table 7).

Analyte/Concentration ng/mL QC1 QC2 QC3

25-Hydroxyvitamin D2 10.0 20.0 30.0 25-Hydroxyvitamin D3 25.1 39.9 60.8

TABLE 7. Matrix Effects *

TABLE 6. System Reproducibility *

TABLE 5. Inter-assay Precision and Accuracy *

TABLE 4. Intra-assay Precision and Accuracy *

021715_APCI_4xP_D1_Cal_7 #752 RT: 1.13 AV: 1 NL: 5.82E6F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00]

50 100 150 200 250 300 350 400m/z

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lativ

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383.3298

365.3195

257.2257

121.1012245.225695.0857 135.1167 159.1164 191.1792 269.2241 309.256669.0704

225.1631

327.2668

Conclusion Method meets clinical research requirements for analysis of Vitamin D

25-hydroxy metabolites in plasma samples.

The calibration range used in method evaluation experiments was 1 to 100 ng/mL, but for improved method robustness, recommended concentration range is 4-100 ng/mL.

Deuterated analog of 25OHD2 is recommended to correct for limited matrix effects we observed during method evaluation.

Purpose To evaluate a rapid quantitative analysis of Vitamin D in human plasma samples using a bench-top quadrupole orbitrap high resolution mass spectrometer for use in clinical research.

Introduction Clinical researchers commonly use a triple quadrupole mass spectrometer for analysis of 25-hydroxyvitamin D2 (25OHD2) and 25-hydroxyvitamin D3 (25OHD3) in plasma. We evaluated the Thermo Scientific™ Q Exactive™

Focus mass spectrometer equipped with Thermo Scientific™ Orbitrap™ technology using a fast, cost-efficient method that collected high resolution MS/MS spectra for improved method specificity. Protein precipitated plasma samples were analyzed with 3 min LC method, and high resolution MS/MS spectra were collected for each analyte. The most abundant fragment, besides water-loss, in each MS2 spectrum was selected for quantitative analysis (Table 3, Figure 1). The linearity range was 4-100 ng/mL (Figure 3, Figure 4); precision and accuracy were within 15%; matrix effects and interferences were not observed.

Instruments LC system

Pump: Thermo Scientific TM Dionex TM Ultimate TM 3000 Autosampler: Thermo Scientific TM OAS-3X00TXRS

Q Exactive Focus orbitrap mass spectrometer

Methods Calibrators

25-hydroxyvitamin D2 (25OHD2), 25-hydroxyvitamin D3 (25OHD3) were purchased from Cerillant Corporation. Since analyte free matrix was not available, calibration standards were prepared in ethanol. NIST controls and spiked plasma recovery data were used to prove calibration curve accuracy.

Sample Preparation

1.100 µL of plasma sample + 300 uL of acetonitrile containing internal standard (25 ng/mL d6-25-hydroxyvitamin D3 ). 2.Vortex, centrifuge 3.Inject 50 µL into LC-MS system.

LC method

Mobile phase A: 0.1% formic acid in water Mobile phase B: 0.1% formic acid in methanol Column: Thermo Scientific TM Hypersil GOLDM aQ 5µ 50x2.1mm

TABLE 1. HPLC Gradient Method

Mass Spectrometry Method

APCI ionization source

Data acquisition method: parallel reaction monitoring (PRM) experiment collecting MS2 spectra for each analyte.

Resolution: 17.5K

Data Analysis

Thermo Scientific™ TraceFinder 3.2 software was used for all data processing and analysis.

Method Performance Evaluation QC samples were prepared by spiking previously analyzed donor plasma to concentrations specified in Table 2 and Figure 2.

TABLE 2. QC Samples Concentrations

Results FIGURE 1. 25OHD2, 25OHD3 MS/MS Spectrum

FIGURE 2. Chromatogram of QC Plasma Samples

QC1 QC2 QC3

25OHD2

25OHD3

6-25OHD3

(IS)

FIGURE 3. Calibration Curves with Lowest Calibration Standard Peaks

25OHD2

4.0 ng/mL

25OHD3

4.0 ng/mL

d6-25OHD3

(IS), 25 ng/mL

©2015 Thermo Fisher Scientific. All Rights Reserved.

All other trademarks are the property of Thermo Fisher Scientific and its subsidiaries.

This information is not intended to encourage use of these products in any manners that might infringe the intellectual property rights of others.

Evaluation of Bench-top Quadrupole Orbitrap Ultra High Resolution MS for Use in Clinical Research in Rapid Quantitative Analysis of Vitamin D in Human Plasma Mindy Gao, Marta Kozak Thermo Fisher Scientific, San Jose, CA, USA

For research use only. Not for use in diagnostic procedures.

Time (min) Flow rate (mL/min) %A (mobile phase) 0 0.70 20 0.2 0.70 20 0.3 0.70 5 1.5 0.70 5 1.6 0.70 20 2.0 0.70 20

021715_APCI_4xP_D1_Cal_7 #787 RT: 1.17 AV: 1 NL: 3.64E6F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00]

50 100 150 200 250 300 350 400m/z

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lativ

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395.3300

377.3193

269.1893

83.0860229.1583119.0856

209.1322251.1792135.1168 159.1163 185.1320 307.2419

279.2106

335.2729

Water lost fragment

Quantifier

25OHD2

Quantifier

Water lost fragment

25OHD3

RT: 0.00 - 2.00 SM: 5B

0.0 0.5 1.0 1.5 2.0Time (min)

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1001.17

1.13

1.13

NL: 7.56E4m/z= 269.1848-269.1948 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_PlasmaL_5

NL: 1.99E5m/z= 257.2214-257.2314 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_PlasmaL_5

NL: 2.07E6m/z= 263.2588-263.2688 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_PlasmaL_5

RT: 0.00 - 2.00 SM: 5B

0.0 0.5 1.0 1.5 2.0Time (min)

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1001.18

1.12

1.12

NL: 1.54E5m/z= 269.1848-269.1948 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_PlasmaM_2

NL: 3.63E5m/z= 257.2214-257.2314 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_PlasmaM_2

NL: 2.65E6m/z= 263.2588-263.2688 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_PlasmaM_2

RT: 0.00 - 2.00 SM: 5B

0.0 0.5 1.0 1.5 2.0Time (min)

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1001.17

1.12

1.12

NL: 2.38E5m/z= 269.1848-269.1948 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_PlasmaH_2

NL: 5.64E5m/z= 257.2214-257.2314 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_PlasmaH_2

NL: 2.62E6m/z= 263.2588-263.2688 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_PlasmaH_2

10.0 ng/mL 30.0 ng/mL 20.0 ng/mL

Collision energy (20 eV) was optimized to maximize response of quantifying fragment ion (m/z=269.1893)

Collision energy (15 eV) was optimized to maximize response of quantifying fragment ion (m/z=257.2257)

25.1 ng/mL 39.9 ng/mL 60.8 ng/mL

4 ng/mL 4 ng/mL

Calculated Amt %Diff 3.98 -0.450 9.97 -0.280 26.1 4.50 50.1 0.120 96.1 -3.88

Calculated Amt %Diff 3.96 -1.10 10.2 1.95 26.3 5.08 46.7 -6.58 101 0.640

Analyte QC1 QC2 QC3 %RSD

25-Hydroxyvitamin D2 6.30 - 12.7 5.33 - 13.0 2.77 - 5.30 25-Hydroxyvitamin D3 3.21 - 7.64 2.64 - 5.89 3.70 - 4.70

%Recovery 25-Hydroxyvitamin D2 87.0 - 100 99.9 - 109 102 - 106 25-Hydroxyvitamin D3 82.9 - 83.5 94.5 - 96.3 91.1 - 101

* 5 replicates of QC samples containing 25OHD2 and 25OHD3 were proceed and analyzed in 3 batches

Analyte QC1 QC2 QC3 %RSD

25-Hydroxyvitamin D2 10.5 9.01 4.51 25-Hydroxyvitamin D3 5.56 3.93 6.1

%Recovery 25-Hydroxyvitamin D2 93.2 105 104 25-Hydroxyvitamin D3 82.9 95.1 97.3

* 5 replicates of QC samples containing 25OHD2 and 25OHD3 were proceed and analyzed in 3 batches

Compound Precursor (m/z)

Quantitation Fragment (m/z)

Collision Energy (V) Polarity

25OHD2 395.3308 269.1898 20 Positive 25OHD3 383.3308 257.2264 15 Positive D6-25OHD3 (IS) 389.3685 263.2638 20 Positive

Analyte Cal-4 Cal-10 Cal-25 Cal-50 Cal-100 %RSD

25OHD2 1.60 2.52 4.27 1.65 2.71 25OHD3 4.72 1.37 4.77 2.01 3.86

%Recovery 25OHD2 99.7 101 96.8 105 96.9 25OHD3 100 101 97.0 98.8 103

* 5 replicate injections of each calibration standard containing 25OHD2 and 25OHD3 were performed to demonstrate the system reproducibility

Analyte Plasma-1 Plasma-2 Plasma-3 Plasma-4 Plasma-5 %RSD

25OHD2 3.65 5.36 9.17 5.90 10.6 25OHD3 2.70 3.48 1.09 4.31 6.99

%Recovery 25OHD2 77.2** 91.7 79.9** 86.5 85.3 25OHD3 112 104 106 109 111

* 15 ng/mL of each analyte was spiked in 5 different plasma samples in 5 replicates

** 25OHD2 % recovery will be increased when deuterated analog will be used as internal standard.

FIGURE 4. Chromatogram of Lowest Calibration Standard

RT: 0.80 - 1.50 SM: 5B

0.8 0.9 1.0 1.1 1.2 1.3 1.4 1.5Time (min)

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1.13

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NL: 2.66E4m/z= 269.1885-269.1911 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_Cal_3

NL: 4.23E4m/z= 257.2251-257.2277 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_Cal_3

NL: 2.24E6m/z= 263.2625-263.2651 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_Cal_3

RT: 0.80 - 1.50 SM: 5B

0.8 0.9 1.0 1.1 1.2 1.3 1.4 1.5Time (min)

0

20

40

60

80

1000

20

40

60

80

100

Relat

ive A

bund

ance

0

20

40

60

80

100 1.18

1.13

1.14

NL: 2.66E4m/z= 269.1885-269.1911 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_Cal_3

NL: 4.23E4m/z= 257.2251-257.2277 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_Cal_3

NL: 2.24E6m/z= 263.2625-263.2651 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_Cal_3

Chromatogram reconstructed with mass accuracy of 5 ppm

System reproducibility was evaluated by analyzing 5 replicates of each calibration standard (Table 6). TABLE 3. PRM transitions of targets and internal standards

Method accuracy was evaluated by obtaining %recovery for NIST controls.

Method precision was evaluated by analyzing 5 replicates of each QC sample in 3 different days (Table 4, Table 5).

Matrix effects were evaluated by spiking previously analyzed plasma from 5 different donors with 25OHD3 and 25OHD2 concentrations of 15 ng/mL and calculating % RSD and % recovery from 5 replicate analysis (Table 7).

Analyte/Concentration ng/mL QC1 QC2 QC3

25-Hydroxyvitamin D2 10.0 20.0 30.0 25-Hydroxyvitamin D3 25.1 39.9 60.8

TABLE 7. Matrix Effects *

TABLE 6. System Reproducibility *

TABLE 5. Inter-assay Precision and Accuracy *

TABLE 4. Intra-assay Precision and Accuracy *

021715_APCI_4xP_D1_Cal_7 #752 RT: 1.13 AV: 1 NL: 5.82E6F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00]

50 100 150 200 250 300 350 400m/z

0

5

10

15

20

25

30

35

40

45

50

55

60

65

70

75

80

85

90

95

100

Re

lativ

e A

bu

nd

an

ce

383.3298

365.3195

257.2257

121.1012245.225695.0857 135.1167 159.1164 191.1792 269.2241 309.256669.0704

225.1631

327.2668

Conclusion Method meets clinical research requirements for analysis of Vitamin D

25-hydroxy metabolites in plasma samples.

The calibration range used in method evaluation experiments was 1 to 100 ng/mL, but for improved method robustness, recommended concentration range is 4-100 ng/mL.

Deuterated analog of 25OHD2 is recommended to correct for limited matrix effects we observed during method evaluation.

Purpose To evaluate a rapid quantitative analysis of Vitamin D in human plasma samples using a bench-top quadrupole orbitrap high resolution mass spectrometer for use in clinical research.

Introduction Clinical researchers commonly use a triple quadrupole mass spectrometer for analysis of 25-hydroxyvitamin D2 (25OHD2) and 25-hydroxyvitamin D3 (25OHD3) in plasma. We evaluated the Thermo Scientific™ Q Exactive™

Focus mass spectrometer equipped with Thermo Scientific™ Orbitrap™ technology using a fast, cost-efficient method that collected high resolution MS/MS spectra for improved method specificity. Protein precipitated plasma samples were analyzed with 3 min LC method, and high resolution MS/MS spectra were collected for each analyte. The most abundant fragment, besides water-loss, in each MS2 spectrum was selected for quantitative analysis (Table 3, Figure 1). The linearity range was 4-100 ng/mL (Figure 3, Figure 4); precision and accuracy were within 15%; matrix effects and interferences were not observed.

Instruments LC system

Pump: Thermo Scientific TM Dionex TM Ultimate TM 3000 Autosampler: Thermo Scientific TM OAS-3X00TXRS

Q Exactive Focus orbitrap mass spectrometer

Methods Calibrators

25-hydroxyvitamin D2 (25OHD2), 25-hydroxyvitamin D3 (25OHD3) were purchased from Cerillant Corporation. Since analyte free matrix was not available, calibration standards were prepared in ethanol. NIST controls and spiked plasma recovery data were used to prove calibration curve accuracy.

Sample Preparation

1.100 µL of plasma sample + 300 uL of acetonitrile containing internal standard (25 ng/mL d6-25-hydroxyvitamin D3 ). 2.Vortex, centrifuge 3.Inject 50 µL into LC-MS system.

LC method

Mobile phase A: 0.1% formic acid in water Mobile phase B: 0.1% formic acid in methanol Column: Thermo Scientific TM Hypersil GOLDM aQ 5µ 50x2.1mm

TABLE 1. HPLC Gradient Method

Mass Spectrometry Method

APCI ionization source

Data acquisition method: parallel reaction monitoring (PRM) experiment collecting MS2 spectra for each analyte.

Resolution: 17.5K

Data Analysis

Thermo Scientific™ TraceFinder 3.2 software was used for all data processing and analysis.

Method Performance Evaluation QC samples were prepared by spiking previously analyzed donor plasma to concentrations specified in Table 2 and Figure 2.

TABLE 2. QC Samples Concentrations

Results FIGURE 1. 25OHD2, 25OHD3 MS/MS Spectrum

FIGURE 2. Chromatogram of QC Plasma Samples

QC1 QC2 QC3

25OHD2

25OHD3

6-25OHD3

(IS)

FIGURE 3. Calibration Curves with Lowest Calibration Standard Peaks

25OHD2

4.0 ng/mL

25OHD3

4.0 ng/mL

d6-25OHD3

(IS), 25 ng/mL

©2015 Thermo Fisher Scientific. All Rights Reserved.

All other trademarks are the property of Thermo Fisher Scientific and its subsidiaries.

This information is not intended to encourage use of these products in any manners that might infringe the intellectual property rights of others.

Evaluation of Bench-top Quadrupole Orbitrap Ultra High Resolution MS for Use in Clinical Research in Rapid Quantitative Analysis of Vitamin D in Human Plasma Mindy Gao, Marta Kozak Thermo Fisher Scientific, San Jose, CA, USA

For research use only. Not for use in diagnostic procedures.

Time (min) Flow rate (mL/min) %A (mobile phase) 0 0.70 20 0.2 0.70 20 0.3 0.70 5 1.5 0.70 5 1.6 0.70 20 2.0 0.70 20

021715_APCI_4xP_D1_Cal_7 #787 RT: 1.17 AV: 1 NL: 3.64E6F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00]

50 100 150 200 250 300 350 400m/z

0

5

10

15

20

25

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35

40

45

50

55

60

65

70

75

80

85

90

95

100

Re

lativ

e A

bu

nd

an

ce

395.3300

377.3193

269.1893

83.0860229.1583119.0856

209.1322251.1792135.1168 159.1163 185.1320 307.2419

279.2106

335.2729

Water lost fragment

Quantifier

25OHD2

Quantifier

Water lost fragment

25OHD3

RT: 0.00 - 2.00 SM: 5B

0.0 0.5 1.0 1.5 2.0Time (min)

0

10

20

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60

70

80

90

1000

10

20

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ce

0

10

20

30

40

50

60

70

80

90

1001.17

1.13

1.13

NL: 7.56E4m/z= 269.1848-269.1948 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_PlasmaL_5

NL: 1.99E5m/z= 257.2214-257.2314 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_PlasmaL_5

NL: 2.07E6m/z= 263.2588-263.2688 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_PlasmaL_5

RT: 0.00 - 2.00 SM: 5B

0.0 0.5 1.0 1.5 2.0Time (min)

0

10

20

30

40

50

60

70

80

90

1000

10

20

30

40

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80

90

100

Re

lativ

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bu

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0

10

20

30

40

50

60

70

80

90

1001.18

1.12

1.12

NL: 1.54E5m/z= 269.1848-269.1948 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_PlasmaM_2

NL: 3.63E5m/z= 257.2214-257.2314 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_PlasmaM_2

NL: 2.65E6m/z= 263.2588-263.2688 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_PlasmaM_2

RT: 0.00 - 2.00 SM: 5B

0.0 0.5 1.0 1.5 2.0Time (min)

0

10

20

30

40

50

60

70

80

90

1000

10

20

30

40

50

60

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80

90

100

Rel

ativ

e A

bund

ance

0

10

20

30

40

50

60

70

80

90

1001.17

1.12

1.12

NL: 2.38E5m/z= 269.1848-269.1948 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_PlasmaH_2

NL: 5.64E5m/z= 257.2214-257.2314 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_PlasmaH_2

NL: 2.62E6m/z= 263.2588-263.2688 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_PlasmaH_2

10.0 ng/mL 30.0 ng/mL 20.0 ng/mL

Collision energy (20 eV) was optimized to maximize response of quantifying fragment ion (m/z=269.1893)

Collision energy (15 eV) was optimized to maximize response of quantifying fragment ion (m/z=257.2257)

25.1 ng/mL 39.9 ng/mL 60.8 ng/mL

4 ng/mL 4 ng/mL

Calculated Amt %Diff 3.98 -0.450 9.97 -0.280 26.1 4.50 50.1 0.120 96.1 -3.88

Calculated Amt %Diff 3.96 -1.10 10.2 1.95 26.3 5.08 46.7 -6.58 101 0.640

Analyte QC1 QC2 QC3 %RSD

25-Hydroxyvitamin D2 6.30 - 12.7 5.33 - 13.0 2.77 - 5.30 25-Hydroxyvitamin D3 3.21 - 7.64 2.64 - 5.89 3.70 - 4.70

%Recovery 25-Hydroxyvitamin D2 87.0 - 100 99.9 - 109 102 - 106 25-Hydroxyvitamin D3 82.9 - 83.5 94.5 - 96.3 91.1 - 101

* 5 replicates of QC samples containing 25OHD2 and 25OHD3 were proceed and analyzed in 3 batches

Analyte QC1 QC2 QC3 %RSD

25-Hydroxyvitamin D2 10.5 9.01 4.51 25-Hydroxyvitamin D3 5.56 3.93 6.1

%Recovery 25-Hydroxyvitamin D2 93.2 105 104 25-Hydroxyvitamin D3 82.9 95.1 97.3

* 5 replicates of QC samples containing 25OHD2 and 25OHD3 were proceed and analyzed in 3 batches

Compound Precursor (m/z)

Quantitation Fragment (m/z)

Collision Energy (V) Polarity

25OHD2 395.3308 269.1898 20 Positive 25OHD3 383.3308 257.2264 15 Positive D6-25OHD3 (IS) 389.3685 263.2638 20 Positive

Analyte Cal-4 Cal-10 Cal-25 Cal-50 Cal-100 %RSD

25OHD2 1.60 2.52 4.27 1.65 2.71 25OHD3 4.72 1.37 4.77 2.01 3.86

%Recovery 25OHD2 99.7 101 96.8 105 96.9 25OHD3 100 101 97.0 98.8 103

* 5 replicate injections of each calibration standard containing 25OHD2 and 25OHD3 were performed to demonstrate the system reproducibility

Analyte Plasma-1 Plasma-2 Plasma-3 Plasma-4 Plasma-5 %RSD

25OHD2 3.65 5.36 9.17 5.90 10.6 25OHD3 2.70 3.48 1.09 4.31 6.99

%Recovery 25OHD2 77.2** 91.7 79.9** 86.5 85.3 25OHD3 112 104 106 109 111

* 15 ng/mL of each analyte was spiked in 5 different plasma samples in 5 replicates

** 25OHD2 % recovery will be increased when deuterated analog will be used as internal standard.

FIGURE 4. Chromatogram of Lowest Calibration Standard

RT: 0.80 - 1.50 SM: 5B

0.8 0.9 1.0 1.1 1.2 1.3 1.4 1.5Time (min)

0

20

40

60

80

1000

20

40

60

80

100

Rela

tive

Abun

danc

e

0

20

40

60

80

100 1.18

1.13

1.14

NL: 2.66E4m/z= 269.1885-269.1911 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_Cal_3

NL: 4.23E4m/z= 257.2251-257.2277 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_Cal_3

NL: 2.24E6m/z= 263.2625-263.2651 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_Cal_3

RT: 0.80 - 1.50 SM: 5B

0.8 0.9 1.0 1.1 1.2 1.3 1.4 1.5Time (min)

0

20

40

60

80

1000

20

40

60

80

100

Relat

ive A

bund

ance

0

20

40

60

80

100 1.18

1.13

1.14

NL: 2.66E4m/z= 269.1885-269.1911 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_Cal_3

NL: 4.23E4m/z= 257.2251-257.2277 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_Cal_3

NL: 2.24E6m/z= 263.2625-263.2651 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_Cal_3

Chromatogram reconstructed with mass accuracy of 5 ppm

System reproducibility was evaluated by analyzing 5 replicates of each calibration standard (Table 6). TABLE 3. PRM transitions of targets and internal standards

Method accuracy was evaluated by obtaining %recovery for NIST controls.

Method precision was evaluated by analyzing 5 replicates of each QC sample in 3 different days (Table 4, Table 5).

Matrix effects were evaluated by spiking previously analyzed plasma from 5 different donors with 25OHD3 and 25OHD2 concentrations of 15 ng/mL and calculating % RSD and % recovery from 5 replicate analysis (Table 7).

Analyte/Concentration ng/mL QC1 QC2 QC3

25-Hydroxyvitamin D2 10.0 20.0 30.0 25-Hydroxyvitamin D3 25.1 39.9 60.8

TABLE 7. Matrix Effects *

TABLE 6. System Reproducibility *

TABLE 5. Inter-assay Precision and Accuracy *

3Thermo Scientific Poster Note • MASCL • PN64374-EN 0315S

TABLE 4. Intra-assay Precision and Accuracy *

021715_APCI_4xP_D1_Cal_7 #752 RT: 1.13 AV: 1 NL: 5.82E6F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00]

50 100 150 200 250 300 350 400m/z

0

5

10

15

20

25

30

35

40

45

50

55

60

65

70

75

80

85

90

95

100

Re

lativ

e A

bu

nd

an

ce

383.3298

365.3195

257.2257

121.1012245.225695.0857 135.1167 159.1164 191.1792 269.2241 309.256669.0704

225.1631

327.2668

Conclusion Method meets clinical research requirements for analysis of Vitamin D

25-hydroxy metabolites in plasma samples.

The calibration range used in method evaluation experiments was 1 to 100 ng/mL, but for improved method robustness, recommended concentration range is 4-100 ng/mL.

Deuterated analog of 25OHD2 is recommended to correct for limited matrix effects we observed during method evaluation.

Purpose To evaluate a rapid quantitative analysis of Vitamin D in human plasma samples using a bench-top quadrupole orbitrap high resolution mass spectrometer for use in clinical research.

Introduction Clinical researchers commonly use a triple quadrupole mass spectrometer for analysis of 25-hydroxyvitamin D2 (25OHD2) and 25-hydroxyvitamin D3 (25OHD3) in plasma. We evaluated the Thermo Scientific™ Q Exactive™

Focus mass spectrometer equipped with Thermo Scientific™ Orbitrap™ technology using a fast, cost-efficient method that collected high resolution MS/MS spectra for improved method specificity. Protein precipitated plasma samples were analyzed with 3 min LC method, and high resolution MS/MS spectra were collected for each analyte. The most abundant fragment, besides water-loss, in each MS2 spectrum was selected for quantitative analysis (Table 3, Figure 1). The linearity range was 4-100 ng/mL (Figure 3, Figure 4); precision and accuracy were within 15%; matrix effects and interferences were not observed.

Instruments LC system

Pump: Thermo Scientific TM Dionex TM Ultimate TM 3000 Autosampler: Thermo Scientific TM OAS-3X00TXRS

Q Exactive Focus orbitrap mass spectrometer

Methods Calibrators

25-hydroxyvitamin D2 (25OHD2), 25-hydroxyvitamin D3 (25OHD3) were purchased from Cerillant Corporation. Since analyte free matrix was not available, calibration standards were prepared in ethanol. NIST controls and spiked plasma recovery data were used to prove calibration curve accuracy.

Sample Preparation

1.100 µL of plasma sample + 300 uL of acetonitrile containing internal standard (25 ng/mL d6-25-hydroxyvitamin D3 ). 2.Vortex, centrifuge 3.Inject 50 µL into LC-MS system.

LC method

Mobile phase A: 0.1% formic acid in water Mobile phase B: 0.1% formic acid in methanol Column: Thermo Scientific TM Hypersil GOLDM aQ 5µ 50x2.1mm

TABLE 1. HPLC Gradient Method

Mass Spectrometry Method

APCI ionization source

Data acquisition method: parallel reaction monitoring (PRM) experiment collecting MS2 spectra for each analyte.

Resolution: 17.5K

Data Analysis

Thermo Scientific™ TraceFinder 3.2 software was used for all data processing and analysis.

Method Performance Evaluation QC samples were prepared by spiking previously analyzed donor plasma to concentrations specified in Table 2 and Figure 2.

TABLE 2. QC Samples Concentrations

Results FIGURE 1. 25OHD2, 25OHD3 MS/MS Spectrum

FIGURE 2. Chromatogram of QC Plasma Samples

QC1 QC2 QC3

25OHD2

25OHD3

6-25OHD3

(IS)

FIGURE 3. Calibration Curves with Lowest Calibration Standard Peaks

25OHD2

4.0 ng/mL

25OHD3

4.0 ng/mL

d6-25OHD3

(IS), 25 ng/mL

©2015 Thermo Fisher Scientific. All Rights Reserved.

All other trademarks are the property of Thermo Fisher Scientific and its subsidiaries.

This information is not intended to encourage use of these products in any manners that might infringe the intellectual property rights of others.

Evaluation of Bench-top Quadrupole Orbitrap Ultra High Resolution MS for Use in Clinical Research in Rapid Quantitative Analysis of Vitamin D in Human Plasma Mindy Gao, Marta Kozak Thermo Fisher Scientific, San Jose, CA, USA

For research use only. Not for use in diagnostic procedures.

Time (min) Flow rate (mL/min) %A (mobile phase) 0 0.70 20 0.2 0.70 20 0.3 0.70 5 1.5 0.70 5 1.6 0.70 20 2.0 0.70 20

021715_APCI_4xP_D1_Cal_7 #787 RT: 1.17 AV: 1 NL: 3.64E6F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00]

50 100 150 200 250 300 350 400m/z

0

5

10

15

20

25

30

35

40

45

50

55

60

65

70

75

80

85

90

95

100

Re

lativ

e A

bu

nd

an

ce

395.3300

377.3193

269.1893

83.0860229.1583119.0856

209.1322251.1792135.1168 159.1163 185.1320 307.2419

279.2106

335.2729

Water lost fragment

Quantifier

25OHD2

Quantifier

Water lost fragment

25OHD3

RT: 0.00 - 2.00 SM: 5B

0.0 0.5 1.0 1.5 2.0Time (min)

0

10

20

30

40

50

60

70

80

90

1000

10

20

30

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0

10

20

30

40

50

60

70

80

90

1001.17

1.13

1.13

NL: 7.56E4m/z= 269.1848-269.1948 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_PlasmaL_5

NL: 1.99E5m/z= 257.2214-257.2314 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_PlasmaL_5

NL: 2.07E6m/z= 263.2588-263.2688 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_PlasmaL_5

RT: 0.00 - 2.00 SM: 5B

0.0 0.5 1.0 1.5 2.0Time (min)

0

10

20

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40

50

60

70

80

90

1000

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0

10

20

30

40

50

60

70

80

90

1001.18

1.12

1.12

NL: 1.54E5m/z= 269.1848-269.1948 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_PlasmaM_2

NL: 3.63E5m/z= 257.2214-257.2314 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_PlasmaM_2

NL: 2.65E6m/z= 263.2588-263.2688 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_PlasmaM_2

RT: 0.00 - 2.00 SM: 5B

0.0 0.5 1.0 1.5 2.0Time (min)

0

10

20

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60

70

80

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100

Rel

ativ

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bund

ance

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10

20

30

40

50

60

70

80

90

1001.17

1.12

1.12

NL: 2.38E5m/z= 269.1848-269.1948 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_PlasmaH_2

NL: 5.64E5m/z= 257.2214-257.2314 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_PlasmaH_2

NL: 2.62E6m/z= 263.2588-263.2688 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_PlasmaH_2

10.0 ng/mL 30.0 ng/mL 20.0 ng/mL

Collision energy (20 eV) was optimized to maximize response of quantifying fragment ion (m/z=269.1893)

Collision energy (15 eV) was optimized to maximize response of quantifying fragment ion (m/z=257.2257)

25.1 ng/mL 39.9 ng/mL 60.8 ng/mL

4 ng/mL 4 ng/mL

Calculated Amt %Diff 3.98 -0.450 9.97 -0.280 26.1 4.50 50.1 0.120 96.1 -3.88

Calculated Amt %Diff 3.96 -1.10 10.2 1.95 26.3 5.08 46.7 -6.58 101 0.640

Analyte QC1 QC2 QC3 %RSD

25-Hydroxyvitamin D2 6.30 - 12.7 5.33 - 13.0 2.77 - 5.30 25-Hydroxyvitamin D3 3.21 - 7.64 2.64 - 5.89 3.70 - 4.70

%Recovery 25-Hydroxyvitamin D2 87.0 - 100 99.9 - 109 102 - 106 25-Hydroxyvitamin D3 82.9 - 83.5 94.5 - 96.3 91.1 - 101

* 5 replicates of QC samples containing 25OHD2 and 25OHD3 were proceed and analyzed in 3 batches

Analyte QC1 QC2 QC3 %RSD

25-Hydroxyvitamin D2 10.5 9.01 4.51 25-Hydroxyvitamin D3 5.56 3.93 6.1

%Recovery 25-Hydroxyvitamin D2 93.2 105 104 25-Hydroxyvitamin D3 82.9 95.1 97.3

* 5 replicates of QC samples containing 25OHD2 and 25OHD3 were proceed and analyzed in 3 batches

Compound Precursor (m/z)

Quantitation Fragment (m/z)

Collision Energy (V) Polarity

25OHD2 395.3308 269.1898 20 Positive 25OHD3 383.3308 257.2264 15 Positive D6-25OHD3 (IS) 389.3685 263.2638 20 Positive

Analyte Cal-4 Cal-10 Cal-25 Cal-50 Cal-100 %RSD

25OHD2 1.60 2.52 4.27 1.65 2.71 25OHD3 4.72 1.37 4.77 2.01 3.86

%Recovery 25OHD2 99.7 101 96.8 105 96.9 25OHD3 100 101 97.0 98.8 103

* 5 replicate injections of each calibration standard containing 25OHD2 and 25OHD3 were performed to demonstrate the system reproducibility

Analyte Plasma-1 Plasma-2 Plasma-3 Plasma-4 Plasma-5 %RSD

25OHD2 3.65 5.36 9.17 5.90 10.6 25OHD3 2.70 3.48 1.09 4.31 6.99

%Recovery 25OHD2 77.2** 91.7 79.9** 86.5 85.3 25OHD3 112 104 106 109 111

* 15 ng/mL of each analyte was spiked in 5 different plasma samples in 5 replicates

** 25OHD2 % recovery will be increased when deuterated analog will be used as internal standard.

FIGURE 4. Chromatogram of Lowest Calibration Standard

RT: 0.80 - 1.50 SM: 5B

0.8 0.9 1.0 1.1 1.2 1.3 1.4 1.5Time (min)

0

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Rela

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Abun

danc

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0

20

40

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100 1.18

1.13

1.14

NL: 2.66E4m/z= 269.1885-269.1911 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_Cal_3

NL: 4.23E4m/z= 257.2251-257.2277 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_Cal_3

NL: 2.24E6m/z= 263.2625-263.2651 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_Cal_3

RT: 0.80 - 1.50 SM: 5B

0.8 0.9 1.0 1.1 1.2 1.3 1.4 1.5Time (min)

0

20

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20

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ive A

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0

20

40

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100 1.18

1.13

1.14

NL: 2.66E4m/z= 269.1885-269.1911 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_Cal_3

NL: 4.23E4m/z= 257.2251-257.2277 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_Cal_3

NL: 2.24E6m/z= 263.2625-263.2651 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_Cal_3

Chromatogram reconstructed with mass accuracy of 5 ppm

System reproducibility was evaluated by analyzing 5 replicates of each calibration standard (Table 6). TABLE 3. PRM transitions of targets and internal standards

Method accuracy was evaluated by obtaining %recovery for NIST controls.

Method precision was evaluated by analyzing 5 replicates of each QC sample in 3 different days (Table 4, Table 5).

Matrix effects were evaluated by spiking previously analyzed plasma from 5 different donors with 25OHD3 and 25OHD2 concentrations of 15 ng/mL and calculating % RSD and % recovery from 5 replicate analysis (Table 7).

Analyte/Concentration ng/mL QC1 QC2 QC3

25-Hydroxyvitamin D2 10.0 20.0 30.0 25-Hydroxyvitamin D3 25.1 39.9 60.8

TABLE 7. Matrix Effects *

TABLE 6. System Reproducibility *

TABLE 5. Inter-assay Precision and Accuracy *

TABLE 4. Intra-assay Precision and Accuracy *

021715_APCI_4xP_D1_Cal_7 #752 RT: 1.13 AV: 1 NL: 5.82E6F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00]

50 100 150 200 250 300 350 400m/z

0

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10

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lativ

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383.3298

365.3195

257.2257

121.1012245.225695.0857 135.1167 159.1164 191.1792 269.2241 309.256669.0704

225.1631

327.2668

Conclusion Method meets clinical research requirements for analysis of Vitamin D

25-hydroxy metabolites in plasma samples.

The calibration range used in method evaluation experiments was 1 to 100 ng/mL, but for improved method robustness, recommended concentration range is 4-100 ng/mL.

Deuterated analog of 25OHD2 is recommended to correct for limited matrix effects we observed during method evaluation.

Purpose To evaluate a rapid quantitative analysis of Vitamin D in human plasma samples using a bench-top quadrupole orbitrap high resolution mass spectrometer for use in clinical research.

Introduction Clinical researchers commonly use a triple quadrupole mass spectrometer for analysis of 25-hydroxyvitamin D2 (25OHD2) and 25-hydroxyvitamin D3 (25OHD3) in plasma. We evaluated the Thermo Scientific™ Q Exactive™

Focus mass spectrometer equipped with Thermo Scientific™ Orbitrap™ technology using a fast, cost-efficient method that collected high resolution MS/MS spectra for improved method specificity. Protein precipitated plasma samples were analyzed with 3 min LC method, and high resolution MS/MS spectra were collected for each analyte. The most abundant fragment, besides water-loss, in each MS2 spectrum was selected for quantitative analysis (Table 3, Figure 1). The linearity range was 4-100 ng/mL (Figure 3, Figure 4); precision and accuracy were within 15%; matrix effects and interferences were not observed.

Instruments LC system

Pump: Thermo Scientific TM Dionex TM Ultimate TM 3000 Autosampler: Thermo Scientific TM OAS-3X00TXRS

Q Exactive Focus orbitrap mass spectrometer

Methods Calibrators

25-hydroxyvitamin D2 (25OHD2), 25-hydroxyvitamin D3 (25OHD3) were purchased from Cerillant Corporation. Since analyte free matrix was not available, calibration standards were prepared in ethanol. NIST controls and spiked plasma recovery data were used to prove calibration curve accuracy.

Sample Preparation

1.100 µL of plasma sample + 300 uL of acetonitrile containing internal standard (25 ng/mL d6-25-hydroxyvitamin D3 ). 2.Vortex, centrifuge 3.Inject 50 µL into LC-MS system.

LC method

Mobile phase A: 0.1% formic acid in water Mobile phase B: 0.1% formic acid in methanol Column: Thermo Scientific TM Hypersil GOLDM aQ 5µ 50x2.1mm

TABLE 1. HPLC Gradient Method

Mass Spectrometry Method

APCI ionization source

Data acquisition method: parallel reaction monitoring (PRM) experiment collecting MS2 spectra for each analyte.

Resolution: 17.5K

Data Analysis

Thermo Scientific™ TraceFinder 3.2 software was used for all data processing and analysis.

Method Performance Evaluation QC samples were prepared by spiking previously analyzed donor plasma to concentrations specified in Table 2 and Figure 2.

TABLE 2. QC Samples Concentrations

Results FIGURE 1. 25OHD2, 25OHD3 MS/MS Spectrum

FIGURE 2. Chromatogram of QC Plasma Samples

QC1 QC2 QC3

25OHD2

25OHD3

6-25OHD3

(IS)

FIGURE 3. Calibration Curves with Lowest Calibration Standard Peaks

25OHD2

4.0 ng/mL

25OHD3

4.0 ng/mL

d6-25OHD3

(IS), 25 ng/mL

©2015 Thermo Fisher Scientific. All Rights Reserved.

All other trademarks are the property of Thermo Fisher Scientific and its subsidiaries.

This information is not intended to encourage use of these products in any manners that might infringe the intellectual property rights of others.

Evaluation of Bench-top Quadrupole Orbitrap Ultra High Resolution MS for Use in Clinical Research in Rapid Quantitative Analysis of Vitamin D in Human Plasma Mindy Gao, Marta Kozak Thermo Fisher Scientific, San Jose, CA, USA

For research use only. Not for use in diagnostic procedures.

Time (min) Flow rate (mL/min) %A (mobile phase) 0 0.70 20 0.2 0.70 20 0.3 0.70 5 1.5 0.70 5 1.6 0.70 20 2.0 0.70 20

021715_APCI_4xP_D1_Cal_7 #787 RT: 1.17 AV: 1 NL: 3.64E6F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00]

50 100 150 200 250 300 350 400m/z

0

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395.3300

377.3193

269.1893

83.0860229.1583119.0856

209.1322251.1792135.1168 159.1163 185.1320 307.2419

279.2106

335.2729

Water lost fragment

Quantifier

25OHD2

Quantifier

Water lost fragment

25OHD3

RT: 0.00 - 2.00 SM: 5B

0.0 0.5 1.0 1.5 2.0Time (min)

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1001.17

1.13

1.13

NL: 7.56E4m/z= 269.1848-269.1948 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_PlasmaL_5

NL: 1.99E5m/z= 257.2214-257.2314 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_PlasmaL_5

NL: 2.07E6m/z= 263.2588-263.2688 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_PlasmaL_5

RT: 0.00 - 2.00 SM: 5B

0.0 0.5 1.0 1.5 2.0Time (min)

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1001.18

1.12

1.12

NL: 1.54E5m/z= 269.1848-269.1948 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_PlasmaM_2

NL: 3.63E5m/z= 257.2214-257.2314 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_PlasmaM_2

NL: 2.65E6m/z= 263.2588-263.2688 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_PlasmaM_2

RT: 0.00 - 2.00 SM: 5B

0.0 0.5 1.0 1.5 2.0Time (min)

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60

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80

90

1001.17

1.12

1.12

NL: 2.38E5m/z= 269.1848-269.1948 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_PlasmaH_2

NL: 5.64E5m/z= 257.2214-257.2314 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_PlasmaH_2

NL: 2.62E6m/z= 263.2588-263.2688 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_PlasmaH_2

10.0 ng/mL 30.0 ng/mL 20.0 ng/mL

Collision energy (20 eV) was optimized to maximize response of quantifying fragment ion (m/z=269.1893)

Collision energy (15 eV) was optimized to maximize response of quantifying fragment ion (m/z=257.2257)

25.1 ng/mL 39.9 ng/mL 60.8 ng/mL

4 ng/mL 4 ng/mL

Calculated Amt %Diff 3.98 -0.450 9.97 -0.280 26.1 4.50 50.1 0.120 96.1 -3.88

Calculated Amt %Diff 3.96 -1.10 10.2 1.95 26.3 5.08 46.7 -6.58 101 0.640

Analyte QC1 QC2 QC3 %RSD

25-Hydroxyvitamin D2 6.30 - 12.7 5.33 - 13.0 2.77 - 5.30 25-Hydroxyvitamin D3 3.21 - 7.64 2.64 - 5.89 3.70 - 4.70

%Recovery 25-Hydroxyvitamin D2 87.0 - 100 99.9 - 109 102 - 106 25-Hydroxyvitamin D3 82.9 - 83.5 94.5 - 96.3 91.1 - 101

* 5 replicates of QC samples containing 25OHD2 and 25OHD3 were proceed and analyzed in 3 batches

Analyte QC1 QC2 QC3 %RSD

25-Hydroxyvitamin D2 10.5 9.01 4.51 25-Hydroxyvitamin D3 5.56 3.93 6.1

%Recovery 25-Hydroxyvitamin D2 93.2 105 104 25-Hydroxyvitamin D3 82.9 95.1 97.3

* 5 replicates of QC samples containing 25OHD2 and 25OHD3 were proceed and analyzed in 3 batches

Compound Precursor (m/z)

Quantitation Fragment (m/z)

Collision Energy (V) Polarity

25OHD2 395.3308 269.1898 20 Positive 25OHD3 383.3308 257.2264 15 Positive D6-25OHD3 (IS) 389.3685 263.2638 20 Positive

Analyte Cal-4 Cal-10 Cal-25 Cal-50 Cal-100 %RSD

25OHD2 1.60 2.52 4.27 1.65 2.71 25OHD3 4.72 1.37 4.77 2.01 3.86

%Recovery 25OHD2 99.7 101 96.8 105 96.9 25OHD3 100 101 97.0 98.8 103

* 5 replicate injections of each calibration standard containing 25OHD2 and 25OHD3 were performed to demonstrate the system reproducibility

Analyte Plasma-1 Plasma-2 Plasma-3 Plasma-4 Plasma-5 %RSD

25OHD2 3.65 5.36 9.17 5.90 10.6 25OHD3 2.70 3.48 1.09 4.31 6.99

%Recovery 25OHD2 77.2** 91.7 79.9** 86.5 85.3 25OHD3 112 104 106 109 111

* 15 ng/mL of each analyte was spiked in 5 different plasma samples in 5 replicates

** 25OHD2 % recovery will be increased when deuterated analog will be used as internal standard.

FIGURE 4. Chromatogram of Lowest Calibration Standard

RT: 0.80 - 1.50 SM: 5B

0.8 0.9 1.0 1.1 1.2 1.3 1.4 1.5Time (min)

0

20

40

60

80

1000

20

40

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80

100

Rela

tive

Abun

danc

e

0

20

40

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100 1.18

1.13

1.14

NL: 2.66E4m/z= 269.1885-269.1911 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_Cal_3

NL: 4.23E4m/z= 257.2251-257.2277 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_Cal_3

NL: 2.24E6m/z= 263.2625-263.2651 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_Cal_3

RT: 0.80 - 1.50 SM: 5B

0.8 0.9 1.0 1.1 1.2 1.3 1.4 1.5Time (min)

0

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Relat

ive A

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0

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100 1.18

1.13

1.14

NL: 2.66E4m/z= 269.1885-269.1911 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_Cal_3

NL: 4.23E4m/z= 257.2251-257.2277 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_Cal_3

NL: 2.24E6m/z= 263.2625-263.2651 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_Cal_3

Chromatogram reconstructed with mass accuracy of 5 ppm

System reproducibility was evaluated by analyzing 5 replicates of each calibration standard (Table 6). TABLE 3. PRM transitions of targets and internal standards

Method accuracy was evaluated by obtaining %recovery for NIST controls.

Method precision was evaluated by analyzing 5 replicates of each QC sample in 3 different days (Table 4, Table 5).

Matrix effects were evaluated by spiking previously analyzed plasma from 5 different donors with 25OHD3 and 25OHD2 concentrations of 15 ng/mL and calculating % RSD and % recovery from 5 replicate analysis (Table 7).

Analyte/Concentration ng/mL QC1 QC2 QC3

25-Hydroxyvitamin D2 10.0 20.0 30.0 25-Hydroxyvitamin D3 25.1 39.9 60.8

TABLE 7. Matrix Effects *

TABLE 6. System Reproducibility *

TABLE 5. Inter-assay Precision and Accuracy *

TABLE 4. Intra-assay Precision and Accuracy *

021715_APCI_4xP_D1_Cal_7 #752 RT: 1.13 AV: 1 NL: 5.82E6F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00]

50 100 150 200 250 300 350 400m/z

0

5

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15

20

25

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40

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Re

lativ

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bu

nd

an

ce

383.3298

365.3195

257.2257

121.1012245.225695.0857 135.1167 159.1164 191.1792 269.2241 309.256669.0704

225.1631

327.2668

Conclusion Method meets clinical research requirements for analysis of Vitamin D

25-hydroxy metabolites in plasma samples.

The calibration range used in method evaluation experiments was 1 to 100 ng/mL, but for improved method robustness, recommended concentration range is 4-100 ng/mL.

Deuterated analog of 25OHD2 is recommended to correct for limited matrix effects we observed during method evaluation.

Purpose To evaluate a rapid quantitative analysis of Vitamin D in human plasma samples using a bench-top quadrupole orbitrap high resolution mass spectrometer for use in clinical research.

Introduction Clinical researchers commonly use a triple quadrupole mass spectrometer for analysis of 25-hydroxyvitamin D2 (25OHD2) and 25-hydroxyvitamin D3 (25OHD3) in plasma. We evaluated the Thermo Scientific™ Q Exactive™

Focus mass spectrometer equipped with Thermo Scientific™ Orbitrap™ technology using a fast, cost-efficient method that collected high resolution MS/MS spectra for improved method specificity. Protein precipitated plasma samples were analyzed with 3 min LC method, and high resolution MS/MS spectra were collected for each analyte. The most abundant fragment, besides water-loss, in each MS2 spectrum was selected for quantitative analysis (Table 3, Figure 1). The linearity range was 4-100 ng/mL (Figure 3, Figure 4); precision and accuracy were within 15%; matrix effects and interferences were not observed.

Instruments LC system

Pump: Thermo Scientific TM Dionex TM Ultimate TM 3000 Autosampler: Thermo Scientific TM OAS-3X00TXRS

Q Exactive Focus orbitrap mass spectrometer

Methods Calibrators

25-hydroxyvitamin D2 (25OHD2), 25-hydroxyvitamin D3 (25OHD3) were purchased from Cerillant Corporation. Since analyte free matrix was not available, calibration standards were prepared in ethanol. NIST controls and spiked plasma recovery data were used to prove calibration curve accuracy.

Sample Preparation

1.100 µL of plasma sample + 300 uL of acetonitrile containing internal standard (25 ng/mL d6-25-hydroxyvitamin D3 ). 2.Vortex, centrifuge 3.Inject 50 µL into LC-MS system.

LC method

Mobile phase A: 0.1% formic acid in water Mobile phase B: 0.1% formic acid in methanol Column: Thermo Scientific TM Hypersil GOLDM aQ 5µ 50x2.1mm

TABLE 1. HPLC Gradient Method

Mass Spectrometry Method

APCI ionization source

Data acquisition method: parallel reaction monitoring (PRM) experiment collecting MS2 spectra for each analyte.

Resolution: 17.5K

Data Analysis

Thermo Scientific™ TraceFinder 3.2 software was used for all data processing and analysis.

Method Performance Evaluation QC samples were prepared by spiking previously analyzed donor plasma to concentrations specified in Table 2 and Figure 2.

TABLE 2. QC Samples Concentrations

Results FIGURE 1. 25OHD2, 25OHD3 MS/MS Spectrum

FIGURE 2. Chromatogram of QC Plasma Samples

QC1 QC2 QC3

25OHD2

25OHD3

6-25OHD3

(IS)

FIGURE 3. Calibration Curves with Lowest Calibration Standard Peaks

25OHD2

4.0 ng/mL

25OHD3

4.0 ng/mL

d6-25OHD3

(IS), 25 ng/mL

©2015 Thermo Fisher Scientific. All Rights Reserved.

All other trademarks are the property of Thermo Fisher Scientific and its subsidiaries.

This information is not intended to encourage use of these products in any manners that might infringe the intellectual property rights of others.

Evaluation of Bench-top Quadrupole Orbitrap Ultra High Resolution MS for Use in Clinical Research in Rapid Quantitative Analysis of Vitamin D in Human Plasma Mindy Gao, Marta Kozak Thermo Fisher Scientific, San Jose, CA, USA

For research use only. Not for use in diagnostic procedures.

Time (min) Flow rate (mL/min) %A (mobile phase) 0 0.70 20 0.2 0.70 20 0.3 0.70 5 1.5 0.70 5 1.6 0.70 20 2.0 0.70 20

021715_APCI_4xP_D1_Cal_7 #787 RT: 1.17 AV: 1 NL: 3.64E6F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00]

50 100 150 200 250 300 350 400m/z

0

5

10

15

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40

45

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55

60

65

70

75

80

85

90

95

100

Re

lativ

e A

bu

nd

an

ce

395.3300

377.3193

269.1893

83.0860229.1583119.0856

209.1322251.1792135.1168 159.1163 185.1320 307.2419

279.2106

335.2729

Water lost fragment

Quantifier

25OHD2

Quantifier

Water lost fragment

25OHD3

RT: 0.00 - 2.00 SM: 5B

0.0 0.5 1.0 1.5 2.0Time (min)

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10

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80

90

1001.17

1.13

1.13

NL: 7.56E4m/z= 269.1848-269.1948 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_PlasmaL_5

NL: 1.99E5m/z= 257.2214-257.2314 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_PlasmaL_5

NL: 2.07E6m/z= 263.2588-263.2688 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_PlasmaL_5

RT: 0.00 - 2.00 SM: 5B

0.0 0.5 1.0 1.5 2.0Time (min)

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1001.18

1.12

1.12

NL: 1.54E5m/z= 269.1848-269.1948 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_PlasmaM_2

NL: 3.63E5m/z= 257.2214-257.2314 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_PlasmaM_2

NL: 2.65E6m/z= 263.2588-263.2688 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_PlasmaM_2

RT: 0.00 - 2.00 SM: 5B

0.0 0.5 1.0 1.5 2.0Time (min)

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1001.17

1.12

1.12

NL: 2.38E5m/z= 269.1848-269.1948 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_PlasmaH_2

NL: 5.64E5m/z= 257.2214-257.2314 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_PlasmaH_2

NL: 2.62E6m/z= 263.2588-263.2688 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_PlasmaH_2

10.0 ng/mL 30.0 ng/mL 20.0 ng/mL

Collision energy (20 eV) was optimized to maximize response of quantifying fragment ion (m/z=269.1893)

Collision energy (15 eV) was optimized to maximize response of quantifying fragment ion (m/z=257.2257)

25.1 ng/mL 39.9 ng/mL 60.8 ng/mL

4 ng/mL 4 ng/mL

Calculated Amt %Diff 3.98 -0.450 9.97 -0.280 26.1 4.50 50.1 0.120 96.1 -3.88

Calculated Amt %Diff 3.96 -1.10 10.2 1.95 26.3 5.08 46.7 -6.58 101 0.640

Analyte QC1 QC2 QC3 %RSD

25-Hydroxyvitamin D2 6.30 - 12.7 5.33 - 13.0 2.77 - 5.30 25-Hydroxyvitamin D3 3.21 - 7.64 2.64 - 5.89 3.70 - 4.70

%Recovery 25-Hydroxyvitamin D2 87.0 - 100 99.9 - 109 102 - 106 25-Hydroxyvitamin D3 82.9 - 83.5 94.5 - 96.3 91.1 - 101

* 5 replicates of QC samples containing 25OHD2 and 25OHD3 were proceed and analyzed in 3 batches

Analyte QC1 QC2 QC3 %RSD

25-Hydroxyvitamin D2 10.5 9.01 4.51 25-Hydroxyvitamin D3 5.56 3.93 6.1

%Recovery 25-Hydroxyvitamin D2 93.2 105 104 25-Hydroxyvitamin D3 82.9 95.1 97.3

* 5 replicates of QC samples containing 25OHD2 and 25OHD3 were proceed and analyzed in 3 batches

Compound Precursor (m/z)

Quantitation Fragment (m/z)

Collision Energy (V) Polarity

25OHD2 395.3308 269.1898 20 Positive 25OHD3 383.3308 257.2264 15 Positive D6-25OHD3 (IS) 389.3685 263.2638 20 Positive

Analyte Cal-4 Cal-10 Cal-25 Cal-50 Cal-100 %RSD

25OHD2 1.60 2.52 4.27 1.65 2.71 25OHD3 4.72 1.37 4.77 2.01 3.86

%Recovery 25OHD2 99.7 101 96.8 105 96.9 25OHD3 100 101 97.0 98.8 103

* 5 replicate injections of each calibration standard containing 25OHD2 and 25OHD3 were performed to demonstrate the system reproducibility

Analyte Plasma-1 Plasma-2 Plasma-3 Plasma-4 Plasma-5 %RSD

25OHD2 3.65 5.36 9.17 5.90 10.6 25OHD3 2.70 3.48 1.09 4.31 6.99

%Recovery 25OHD2 77.2** 91.7 79.9** 86.5 85.3 25OHD3 112 104 106 109 111

* 15 ng/mL of each analyte was spiked in 5 different plasma samples in 5 replicates

** 25OHD2 % recovery will be increased when deuterated analog will be used as internal standard.

FIGURE 4. Chromatogram of Lowest Calibration Standard

RT: 0.80 - 1.50 SM: 5B

0.8 0.9 1.0 1.1 1.2 1.3 1.4 1.5Time (min)

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NL: 2.66E4m/z= 269.1885-269.1911 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_Cal_3

NL: 4.23E4m/z= 257.2251-257.2277 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_Cal_3

NL: 2.24E6m/z= 263.2625-263.2651 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_Cal_3

RT: 0.80 - 1.50 SM: 5B

0.8 0.9 1.0 1.1 1.2 1.3 1.4 1.5Time (min)

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NL: 2.66E4m/z= 269.1885-269.1911 F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00] MS 021715_APCI_4xP_D1_Cal_3

NL: 4.23E4m/z= 257.2251-257.2277 F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00] MS 021715_APCI_4xP_D1_Cal_3

NL: 2.24E6m/z= 263.2625-263.2651 F: FTMS + c APCI corona Full ms2 389.37@hcd20.00 [50.00-415.00] MS 021715_APCI_4xP_D1_Cal_3

Chromatogram reconstructed with mass accuracy of 5 ppm

System reproducibility was evaluated by analyzing 5 replicates of each calibration standard (Table 6). TABLE 3. PRM transitions of targets and internal standards

Method accuracy was evaluated by obtaining %recovery for NIST controls.

Method precision was evaluated by analyzing 5 replicates of each QC sample in 3 different days (Table 4, Table 5).

Matrix effects were evaluated by spiking previously analyzed plasma from 5 different donors with 25OHD3 and 25OHD2 concentrations of 15 ng/mL and calculating % RSD and % recovery from 5 replicate analysis (Table 7).

Analyte/Concentration ng/mL QC1 QC2 QC3

25-Hydroxyvitamin D2 10.0 20.0 30.0 25-Hydroxyvitamin D3 25.1 39.9 60.8

TABLE 7. Matrix Effects *

TABLE 6. System Reproducibility *

TABLE 5. Inter-assay Precision and Accuracy *

Africa +43 1 333 50 34 0Australia +61 3 9757 4300Austria +43 810 282 206Belgium +32 53 73 42 41Brazil +55 11 3731 5140Canada +1 800 530 8447China 800 810 5118 (free call domestic)

400 650 5118

Denmark +45 70 23 62 60Europe-Other +43 1 333 50 34 0Finland +358 9 3291 0200France +33 1 60 92 48 00Germany +49 6103 408 1014India +91 22 6742 9494Italy +39 02 950 591

Japan +81 6 6885 1213Korea +82 2 3420 8600Latin America +1 561 688 8700Middle East +43 1 333 50 34 0Netherlands +31 76 579 55 55 New Zealand +64 9 980 6700 Norway +46 8 556 468 00

Russia/CIS +43 1 333 50 34 0 Singapore +65 6289 1190 Sweden +46 8 556 468 00 Switzerland +41 61 716 77 00 Taiwan +886 2 8751 6655 UK/Ireland +44 1442 233555 USA +1 800 532 4752

PN64374-EN 0616S

www.thermofisher.com©2016 Thermo Fisher Scientific Inc. All rights reserved. All trademarks are the property of Thermo Fisher Scientific and its subsidiaries This information is presented as an example of the capabilities of Thermo Fish

er Scientific products. It is not intended to encourage use of these products

in any manners that might infringe the intellectual property rights of others. Specifications, terms and pricing are subject to change. Not all products are available in all countries. Please consult your local sales representative for details.

For research use only. Not for use in diagnostic procedures.

TABLE 4. Intra-assay Precision and Accuracy *

021715_APCI_4xP_D1_Cal_7 #752 RT: 1.13 AV: 1 NL: 5.82E6F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00]

50 100 150 200 250 300 350 400m/z

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365.3195

257.2257

121.1012245.225695.0857 135.1167 159.1164 191.1792 269.2241 309.256669.0704

225.1631

327.2668

Conclusion Method meets clinical research requirements for analysis of Vitamin D

25-hydroxy metabolites in plasma samples.

The calibration range used in method evaluation experiments was 1 to 100 ng/mL, but for improved method robustness, recommended concentration range is 4-100 ng/mL.

Deuterated analog of 25OHD2 is recommended to correct for limited matrix effects we observed during method evaluation.

PurposeTo evaluate a rapid quantitative analysis of Vitamin D in human plasmasamples using a bench-top quadrupole orbitrap high resolution mass spectrometer for use in clinical research.

IntroductionClinical researchers commonly use a triple quadrupole mass spectrometer for analysis of 25-hydroxyvitamin D2 (25OHD2) and 25-hydroxyvitamin D3 (25OHD3) in plasma. We evaluated the Thermo Scientific™ Q Exactive™Focus mass spectrometer equipped with Thermo Scientific™ Orbitrap™ technology using a fast, cost-efficient method that collected high resolution MS/MS spectra for improved method specificity. Protein precipitated plasma samples were analyzed with 3 min LC method, and high resolution MS/MS spectra were collected for each analyte. The most abundant fragment, besides water-loss, in each MS2 spectrum was selected for quantitative analysis (Table 3, Figure 1). The linearity range was 4-100 ng/mL (Figure 3, Figure 4); precision and accuracy were within 15%; matrix effects and interferences were not observed.

InstrumentsLC system

Pump: Thermo Scientific TM Dionex TM Ultimate TM 3000 Autosampler: Thermo Scientific TM OAS-3X00TXRS

Q Exactive Focus orbitrap mass spectrometer

MethodsCalibrators

25-hydroxyvitamin D2 (25OHD2), 25-hydroxyvitamin D3 (25OHD3) were purchased from Cerillant Corporation. Since analyte free matrix was not available, calibration standards were prepared in ethanol. NIST controls and spiked plasma recovery data were used to prove calibration curve accuracy.

Sample Preparation

1.100 µL of plasma sample + 300 uL of acetonitrile containing internal standard (25 ng/mL d6-25-hydroxyvitamin D3 ).2.Vortex, centrifuge3.Inject 50 µL into LC-MS system.

LC method

Mobile phase A: 0.1% formic acid in water Mobile phase B: 0.1% formic acid in methanolColumn: Thermo Scientific TM Hypersil GOLDM aQ 5µ 50x2.1mm

TABLE 1. HPLC Gradient Method

Mass Spectrometry Method

APCI ionization source

Data acquisition method: parallel reaction monitoring (PRM) experiment collecting MS2 spectra for each analyte.

Resolution: 17.5K

Data Analysis

Thermo Scientific™ TraceFinder 3.2 software was used for all dataprocessing and analysis.

Method Performance EvaluationQC samples were prepared by spiking previously analyzed donor plasmato concentrations specified in Table 2 and Figure 2.

TABLE 2. QC Samples Concentrations

ResultsFIGURE 1. 25OHD2, 25OHD3 MS/MS Spectrum

FIGURE 2. Chromatogram of QC Plasma Samples

QC1 QC2 QC3

25OHD2

25OHD3

6-25OHD3

(IS)

FIGURE 3. Calibration Curves with Lowest Calibration Standard Peaks

25OHD2

4.0 ng/mL

25OHD3

4.0 ng/mL

d6-25OHD3

(IS), 25 ng/mL

©2015 Thermo Fisher Scientific. All Rights Reserved.

All other trademarks are the property of Thermo Fisher Scientific and its subsidiaries.

This information is not intended to encourage use of these products in any manners that might infringe the intellectual property rights of others.

Evaluation of Bench-top Quadrupole Orbitrap Ultra High Resolution MS for Use in Clinical Research in Rapid Quantitative Analysis of Vitamin D in Human PlasmaMindy Gao, Marta KozakThermo Fisher Scientific, San Jose, CA, USA

For research use only. Not for use in diagnostic procedures.

Time (min) Flow rate (mL/min) %A (mobile phase)0 0.70 200.2 0.70 200.3 0.70 51.5 0.70 51.6 0.70 202.0 0.70 20

021715_APCI_4xP_D1_Cal_7 #787 RT: 1.17 AV: 1 NL: 3.64E6F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00]

50 100 150 200 250 300 350 400m/z

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395.3300

377.3193

269.1893

83.0860229.1583119.0856

209.1322251.1792135.1168 159.1163 185.1320 307.2419

279.2106

335.2729

Water lost fragment

Quantifier

25OHD2

Quantifier

Water lost fragment

25OHD3

RT: 0.00 - 2.00 SM: 5B

0.0 0.5 1.0 1.5 2.0Time (min)

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NL: 7.56E4m/z= 269.1848-269.1948 F:FTMS + c APCI corona Fullms2 395.33@hcd20.00 [50.00-420.00] MS021715_APCI_4xP_D1_PlasmaL_5

NL: 1.99E5m/z= 257.2214-257.2314 F:FTMS + c APCI corona Fullms2 383.33@hcd15.00 [50.00-410.00] MS021715_APCI_4xP_D1_PlasmaL_5

NL: 2.07E6m/z= 263.2588-263.2688 F:FTMS + c APCI corona Fullms2 389.37@hcd20.00 [50.00-415.00] MS021715_APCI_4xP_D1_PlasmaL_5

RT: 0.00 - 2.00 SM: 5B

0.0 0.5 1.0 1.5 2.0Time (min)

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1.12

1.12

NL: 1.54E5m/z= 269.1848-269.1948 F:FTMS + c APCI corona Fullms2 395.33@hcd20.00 [50.00-420.00] MS021715_APCI_4xP_D1_PlasmaM_2

NL: 3.63E5m/z= 257.2214-257.2314 F:FTMS + c APCI corona Fullms2 383.33@hcd15.00 [50.00-410.00] MS021715_APCI_4xP_D1_PlasmaM_2

NL: 2.65E6m/z= 263.2588-263.2688 F:FTMS + c APCI corona Fullms2 389.37@hcd20.00 [50.00-415.00] MS021715_APCI_4xP_D1_PlasmaM_2

RT: 0.00 - 2.00 SM: 5B

0.0 0.5 1.0 1.5 2.0Time (min)

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1001.17

1.12

1.12

NL: 2.38E5m/z= 269.1848-269.1948 F:FTMS + c APCI corona Fullms2 395.33@hcd20.00 [50.00-420.00] MS021715_APCI_4xP_D1_PlasmaH_2

NL: 5.64E5m/z= 257.2214-257.2314 F:FTMS + c APCI corona Fullms2 383.33@hcd15.00 [50.00-410.00] MS021715_APCI_4xP_D1_PlasmaH_2

NL: 2.62E6m/z= 263.2588-263.2688 F:FTMS + c APCI corona Fullms2 389.37@hcd20.00 [50.00-415.00] MS021715_APCI_4xP_D1_PlasmaH_2

10.0 ng/mL 30.0 ng/mL20.0 ng/mL

Collision energy (20 eV) was optimized to maximize response of quantifying fragment ion (m/z=269.1893)

Collision energy (15 eV) was optimized to maximize response of quantifying fragment ion (m/z=257.2257)

25.1 ng/mL 39.9 ng/mL 60.8 ng/mL

4 ng/mL 4 ng/mL

Calculated Amt %Diff3.98 -0.4509.97 -0.28026.1 4.5050.1 0.12096.1 -3.88

Calculated Amt %Diff3.96 -1.1010.2 1.9526.3 5.0846.7 -6.58101 0.640

Analyte QC1 QC2 QC3 %RSD

25-Hydroxyvitamin D2 6.30 - 12.7 5.33 - 13.0 2.77 - 5.30 25-Hydroxyvitamin D3 3.21 - 7.64 2.64 - 5.89 3.70 - 4.70

%Recovery 25-Hydroxyvitamin D2 87.0 - 100 99.9 - 109 102 - 106 25-Hydroxyvitamin D3 82.9 - 83.5 94.5 - 96.3 91.1 - 101

* 5 replicates of QC samples containing 25OHD2 and 25OHD3 were proceed and analyzed in 3 batches

Analyte QC1 QC2 QC3 %RSD

25-Hydroxyvitamin D2 10.5 9.01 4.51 25-Hydroxyvitamin D3 5.56 3.93 6.1

%Recovery 25-Hydroxyvitamin D2 93.2 105 104 25-Hydroxyvitamin D3 82.9 95.1 97.3

* 5 replicates of QC samples containing 25OHD2 and 25OHD3 were proceed and analyzed in 3 batches

Compound Precursor (m/z)

Quantitation Fragment (m/z)

Collision Energy (V) Polarity

25OHD2 395.3308 269.1898 20 Positive25OHD3 383.3308 257.2264 15 PositiveD6-25OHD3 (IS) 389.3685 263.2638 20 Positive

Analyte Cal-4 Cal-10 Cal-25 Cal-50 Cal-100 %RSD

25OHD2 1.60 2.52 4.27 1.65 2.71 25OHD3 4.72 1.37 4.77 2.01 3.86

%Recovery 25OHD2 99.7 101 96.8 105 96.9 25OHD3 100 101 97.0 98.8 103

* 5 replicate injections of each calibration standard containing 25OHD2 and 25OHD3 were performed to demonstrate the system reproducibility

Analyte Plasma-1 Plasma-2 Plasma-3 Plasma-4 Plasma-5%RSD

25OHD2 3.65 5.36 9.17 5.90 10.625OHD3 2.70 3.48 1.09 4.31 6.99

%Recovery 25OHD2 77.2** 91.7 79.9** 86.5 85.325OHD3 112 104 106 109 111

* 15 ng/mL of each analyte was spiked in 5 different plasma samples in 5 replicates

** 25OHD2 % recovery will be increased when deuterated analog will be used as internal standard.

FIGURE 4. Chromatogram of Lowest Calibration Standard

RT: 0.80 - 1.50 SM: 5B

0.8 0.9 1.0 1.1 1.2 1.3 1.4 1.5Time (min)

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Rela

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NL: 2.66E4m/z= 269.1885-269.1911 F:FTMS + c APCI corona Fullms2 395.33@hcd20.00 [50.00-420.00] MS021715_APCI_4xP_D1_Cal_3

NL: 4.23E4m/z= 257.2251-257.2277 F:FTMS + c APCI corona Fullms2 383.33@hcd15.00 [50.00-410.00] MS021715_APCI_4xP_D1_Cal_3

NL: 2.24E6m/z= 263.2625-263.2651 F:FTMS + c APCI corona Fullms2 389.37@hcd20.00 [50.00-415.00] MS021715_APCI_4xP_D1_Cal_3

RT: 0.80 - 1.50 SM: 5B

0.8 0.9 1.0 1.1 1.2 1.3 1.4 1.5Time (min)

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NL: 2.66E4m/z= 269.1885-269.1911 F:FTMS + c APCI corona Fullms2 395.33@hcd20.00 [50.00-420.00] MS021715_APCI_4xP_D1_Cal_3

NL: 4.23E4m/z= 257.2251-257.2277 F:FTMS + c APCI corona Fullms2 383.33@hcd15.00 [50.00-410.00] MS021715_APCI_4xP_D1_Cal_3

NL: 2.24E6m/z= 263.2625-263.2651 F:FTMS + c APCI corona Fullms2 389.37@hcd20.00 [50.00-415.00] MS021715_APCI_4xP_D1_Cal_3

Chromatogram reconstructed with mass accuracy of 5 ppm

System reproducibility was evaluated by analyzing 5 replicates of eachcalibration standard (Table 6).

TABLE 3. PRM transitions of targets and internal standards

Method accuracy was evaluated by obtaining %recovery for NIST controls.

Method precision was evaluated by analyzing 5 replicates of each QC sample in 3 different days (Table 4, Table 5).

Matrix effects were evaluated by spiking previously analyzed plasma from 5 different donors with 25OHD3 and 25OHD2 concentrations of 15 ng/mLand calculating % RSD and % recovery from 5 replicate analysis (Table 7).

Analyte/Concentrationng/mL QC1 QC2 QC3

25-Hydroxyvitamin D2 10.0 20.0 30.025-Hydroxyvitamin D3 25.1 39.9 60.8

TABLE 7. Matrix Effects *

TABLE 6. System Reproducibility *

TABLE 5. Inter-assay Precision and Accuracy *

TABLE 4. Intra-assay Precision and Accuracy *

021715_APCI_4xP_D1_Cal_7 #752 RT: 1.13 AV: 1 NL: 5.82E6F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00]

50 100 150 200 250 300 350 400m/z

0

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383.3298

365.3195

257.2257

121.1012245.225695.0857 135.1167 159.1164 191.1792 269.2241 309.256669.0704

225.1631

327.2668

Conclusion Method meets clinical research requirements for analysis of Vitamin D

25-hydroxy metabolites in plasma samples.

The calibration range used in method evaluation experiments was 1 to 100 ng/mL, but for improved method robustness, recommended concentration range is 4-100 ng/mL.

Deuterated analog of 25OHD2 is recommended to correct for limited matrix effects we observed during method evaluation.

PurposeTo evaluate a rapid quantitative analysis of Vitamin D in human plasmasamples using a bench-top quadrupole orbitrap high resolution mass spectrometer for use in clinical research.

IntroductionClinical researchers commonly use a triple quadrupole mass spectrometer for analysis of 25-hydroxyvitamin D2 (25OHD2) and 25-hydroxyvitamin D3 (25OHD3) in plasma. We evaluated the Thermo Scientific™ Q Exactive™Focus mass spectrometer equipped with Thermo Scientific™ Orbitrap™ technology using a fast, cost-efficient method that collected high resolution MS/MS spectra for improved method specificity. Protein precipitated plasma samples were analyzed with 3 min LC method, and high resolution MS/MS spectra were collected for each analyte. The most abundant fragment, besides water-loss, in each MS2 spectrum was selected for quantitative analysis (Table 3, Figure 1). The linearity range was 4-100 ng/mL (Figure 3, Figure 4); precision and accuracy were within 15%; matrix effects and interferences were not observed.

InstrumentsLC system

Pump: Thermo Scientific TM Dionex TM Ultimate TM 3000 Autosampler: Thermo Scientific TM OAS-3X00TXRS

Q Exactive Focus orbitrap mass spectrometer

MethodsCalibrators

25-hydroxyvitamin D2 (25OHD2), 25-hydroxyvitamin D3 (25OHD3) were purchased from Cerillant Corporation. Since analyte free matrix was not available, calibration standards were prepared in ethanol. NIST controls and spiked plasma recovery data were used to prove calibration curve accuracy.

Sample Preparation

1.100 µL of plasma sample + 300 uL of acetonitrile containing internal standard (25 ng/mL d6-25-hydroxyvitamin D3 ).2.Vortex, centrifuge3.Inject 50 µL into LC-MS system.

LC method

Mobile phase A: 0.1% formic acid in water Mobile phase B: 0.1% formic acid in methanolColumn: Thermo Scientific TM Hypersil GOLDM aQ 5µ 50x2.1mm

TABLE 1. HPLC Gradient Method

Mass Spectrometry Method

APCI ionization source

Data acquisition method: parallel reaction monitoring (PRM) experiment collecting MS2 spectra for each analyte.

Resolution: 17.5K

Data Analysis

Thermo Scientific™ TraceFinder 3.2 software was used for all dataprocessing and analysis.

Method Performance EvaluationQC samples were prepared by spiking previously analyzed donor plasmato concentrations specified in Table 2 and Figure 2.

TABLE 2. QC Samples Concentrations

ResultsFIGURE 1. 25OHD2, 25OHD3 MS/MS Spectrum

FIGURE 2. Chromatogram of QC Plasma Samples

QC1 QC2 QC3

25OHD2

25OHD3

6-25OHD3

(IS)

FIGURE 3. Calibration Curves with Lowest Calibration Standard Peaks

25OHD2

4.0 ng/mL

25OHD3

4.0 ng/mL

d6-25OHD3

(IS), 25 ng/mL

©2015 Thermo Fisher Scientific. All Rights Reserved.

All other trademarks are the property of Thermo Fisher Scientific and its subsidiaries.

This information is not intended to encourage use of these products in any manners that might infringe the intellectual property rights of others.

Evaluation of Bench-top Quadrupole Orbitrap Ultra High Resolution MS for Use in Clinical Research in Rapid Quantitative Analysis of Vitamin D in Human PlasmaMindy Gao, Marta KozakThermo Fisher Scientific, San Jose, CA, USA

For research use only. Not for use in diagnostic procedures.

Time (min) Flow rate (mL/min) %A (mobile phase)0 0.70 200.2 0.70 200.3 0.70 51.5 0.70 51.6 0.70 202.0 0.70 20

021715_APCI_4xP_D1_Cal_7 #787 RT: 1.17 AV: 1 NL: 3.64E6F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00]

50 100 150 200 250 300 350 400m/z

0

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55

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75

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85

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95

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Re

lativ

e A

bu

nd

an

ce

395.3300

377.3193

269.1893

83.0860229.1583119.0856

209.1322251.1792135.1168 159.1163 185.1320 307.2419

279.2106

335.2729

Water lost fragment

Quantifier

25OHD2

Quantifier

Water lost fragment

25OHD3

RT: 0.00 - 2.00 SM: 5B

0.0 0.5 1.0 1.5 2.0Time (min)

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1001.17

1.13

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NL: 7.56E4m/z= 269.1848-269.1948 F:FTMS + c APCI corona Fullms2 395.33@hcd20.00 [50.00-420.00] MS021715_APCI_4xP_D1_PlasmaL_5

NL: 1.99E5m/z= 257.2214-257.2314 F:FTMS + c APCI corona Fullms2 383.33@hcd15.00 [50.00-410.00] MS021715_APCI_4xP_D1_PlasmaL_5

NL: 2.07E6m/z= 263.2588-263.2688 F:FTMS + c APCI corona Fullms2 389.37@hcd20.00 [50.00-415.00] MS021715_APCI_4xP_D1_PlasmaL_5

RT: 0.00 - 2.00 SM: 5B

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NL: 1.54E5m/z= 269.1848-269.1948 F:FTMS + c APCI corona Fullms2 395.33@hcd20.00 [50.00-420.00] MS021715_APCI_4xP_D1_PlasmaM_2

NL: 3.63E5m/z= 257.2214-257.2314 F:FTMS + c APCI corona Fullms2 383.33@hcd15.00 [50.00-410.00] MS021715_APCI_4xP_D1_PlasmaM_2

NL: 2.65E6m/z= 263.2588-263.2688 F:FTMS + c APCI corona Fullms2 389.37@hcd20.00 [50.00-415.00] MS021715_APCI_4xP_D1_PlasmaM_2

RT: 0.00 - 2.00 SM: 5B

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NL: 2.38E5m/z= 269.1848-269.1948 F:FTMS + c APCI corona Fullms2 395.33@hcd20.00 [50.00-420.00] MS021715_APCI_4xP_D1_PlasmaH_2

NL: 5.64E5m/z= 257.2214-257.2314 F:FTMS + c APCI corona Fullms2 383.33@hcd15.00 [50.00-410.00] MS021715_APCI_4xP_D1_PlasmaH_2

NL: 2.62E6m/z= 263.2588-263.2688 F:FTMS + c APCI corona Fullms2 389.37@hcd20.00 [50.00-415.00] MS021715_APCI_4xP_D1_PlasmaH_2

10.0 ng/mL 30.0 ng/mL20.0 ng/mL

Collision energy (20 eV) was optimized to maximize response of quantifying fragment ion (m/z=269.1893)

Collision energy (15 eV) was optimized to maximize response of quantifying fragment ion (m/z=257.2257)

25.1 ng/mL 39.9 ng/mL 60.8 ng/mL

4 ng/mL 4 ng/mL

Calculated Amt %Diff3.98 -0.4509.97 -0.28026.1 4.5050.1 0.12096.1 -3.88

Calculated Amt %Diff3.96 -1.1010.2 1.9526.3 5.0846.7 -6.58101 0.640

Analyte QC1 QC2 QC3%RSD

25-Hydroxyvitamin D2 6.30 - 12.7 5.33 - 13.0 2.77 - 5.3025-Hydroxyvitamin D3 3.21 - 7.64 2.64 - 5.89 3.70 - 4.70

%Recovery25-Hydroxyvitamin D2 87.0 - 100 99.9 - 109 102 - 10625-Hydroxyvitamin D3 82.9 - 83.5 94.5 - 96.3 91.1 - 101

* 5 replicates of QC samples containing 25OHD2 and 25OHD3 were proceed and analyzed in 3 batches

Analyte QC1 QC2 QC3%RSD

25-Hydroxyvitamin D2 10.5 9.01 4.5125-Hydroxyvitamin D3 5.56 3.93 6.1

%Recovery25-Hydroxyvitamin D2 93.2 105 10425-Hydroxyvitamin D3 82.9 95.1 97.3

* 5 replicates of QC samples containing 25OHD2 and 25OHD3 were proceed and analyzed in 3 batches

Compound Precursor (m/z)

Quantitation Fragment (m/z)

Collision Energy (V) Polarity

25OHD2 395.3308 269.1898 20 Positive25OHD3 383.3308 257.2264 15 PositiveD6-25OHD3 (IS) 389.3685 263.2638 20 Positive

Analyte Cal-4 Cal-10 Cal-25 Cal-50 Cal-100%RSD

25OHD2 1.60 2.52 4.27 1.65 2.7125OHD3 4.72 1.37 4.77 2.01 3.86

%Recovery25OHD2 99.7 101 96.8 105 96.925OHD3 100 101 97.0 98.8 103

* 5 replicate injections of each calibration standard containing 25OHD2 and 25OHD3 were performed to demonstrate the system reproducibility

Analyte Plasma-1 Plasma-2 Plasma-3 Plasma-4 Plasma-5 %RSD

25OHD2 3.65 5.36 9.17 5.90 10.6 25OHD3 2.70 3.48 1.09 4.31 6.99

%Recovery 25OHD2 77.2** 91.7 79.9** 86.5 85.3 25OHD3 112 104 106 109 111

* 15 ng/mL of each analyte was spiked in 5 different plasma samples in 5 replicates

** 25OHD2 % recovery will be increased when deuterated analog will be used as internal standard.

FIGURE 4. Chromatogram of Lowest Calibration Standard

RT: 0.80 - 1.50 SM: 5B

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NL: 2.66E4m/z= 269.1885-269.1911 F:FTMS + c APCI corona Fullms2 395.33@hcd20.00 [50.00-420.00] MS021715_APCI_4xP_D1_Cal_3

NL: 4.23E4m/z= 257.2251-257.2277 F:FTMS + c APCI corona Fullms2 383.33@hcd15.00 [50.00-410.00] MS021715_APCI_4xP_D1_Cal_3

NL: 2.24E6m/z= 263.2625-263.2651 F:FTMS + c APCI corona Fullms2 389.37@hcd20.00 [50.00-415.00] MS021715_APCI_4xP_D1_Cal_3

RT: 0.80 - 1.50 SM: 5B

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NL: 4.23E4m/z= 257.2251-257.2277 F:FTMS + c APCI corona Fullms2 383.33@hcd15.00 [50.00-410.00] MS021715_APCI_4xP_D1_Cal_3

NL: 2.24E6m/z= 263.2625-263.2651 F:FTMS + c APCI corona Fullms2 389.37@hcd20.00 [50.00-415.00] MS021715_APCI_4xP_D1_Cal_3

Chromatogram reconstructed with mass accuracy of 5 ppm

System reproducibility was evaluated by analyzing 5 replicates of eachcalibration standard (Table 6).

TABLE 3. PRM transitions of targets and internal standards

Method accuracy was evaluated by obtaining %recovery for NIST controls.

Method precision was evaluated by analyzing 5 replicates of each QC sample in 3 different days (Table 4, Table 5).

Matrix effects were evaluated by spiking previously analyzed plasma from 5 different donors with 25OHD3 and 25OHD2 concentrations of 15 ng/mLand calculating % RSD and % recovery from 5 replicate analysis (Table 7).

Analyte/Concentrationng/mL QC1 QC2 QC3

25-Hydroxyvitamin D2 10.0 20.0 30.025-Hydroxyvitamin D3 25.1 39.9 60.8

TABLE 7. Matrix Effects *

TABLE 6. System Reproducibility *

TABLE 5. Inter-assay Precision and Accuracy *

TABLE 4. Intra-assay Precision and Accuracy *

021715_APCI_4xP_D1_Cal_7 #752 RT: 1.13 AV: 1 NL: 5.82E6F: FTMS + c APCI corona Full ms2 383.33@hcd15.00 [50.00-410.00]

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257.2257

121.1012245.225695.0857 135.1167 159.1164 191.1792 269.2241 309.256669.0704

225.1631

327.2668

Conclusion Method meets clinical research requirements for analysis of Vitamin D

25-hydroxy metabolites in plasma samples.

The calibration range used in method evaluation experiments was 1 to100 ng/mL, but for improved method robustness, recommended concentration range is 4-100 ng/mL.

Deuterated analog of 25OHD2 is recommended to correct for limitedmatrix effects we observed during method evaluation.

PurposeTo evaluate a rapid quantitative analysis of Vitamin D in human plasmasamples using a bench-top quadrupole orbitrap high resolution mass spectrometer for use in clinical research.

IntroductionClinical researchers commonly use a triple quadrupole mass spectrometer for analysis of 25-hydroxyvitamin D2 (25OHD2) and 25-hydroxyvitamin D3 (25OHD3) in plasma. We evaluated the Thermo Scientific™ Q Exactive™Focus mass spectrometer equipped with Thermo Scientific™ Orbitrap™ technology using a fast, cost-efficient method that collected high resolution MS/MS spectra for improved method specificity. Protein precipitated plasma samples were analyzed with 3 min LC method, and high resolution MS/MS spectra were collected for each analyte. The most abundant fragment, besides water-loss, in each MS2 spectrum was selected for quantitative analysis (Table 3, Figure 1). The linearity range was 4-100 ng/mL (Figure 3, Figure 4); precision and accuracy were within 15%; matrix effects and interferences were not observed.

InstrumentsLC system

Pump: Thermo Scientific TM Dionex TM Ultimate TM 3000 Autosampler: Thermo Scientific TM OAS-3X00TXRS

Q Exactive Focus orbitrap mass spectrometer

MethodsCalibrators

25-hydroxyvitamin D2 (25OHD2), 25-hydroxyvitamin D3 (25OHD3) were purchased from Cerillant Corporation. Since analyte free matrix was not available, calibration standards were prepared in ethanol. NIST controls and spiked plasma recovery data were used to prove calibration curve accuracy.

Sample Preparation

1.100 µL of plasma sample + 300 uL of acetonitrile containing internal standard (25 ng/mL d6-25-hydroxyvitamin D3 ).2.Vortex, centrifuge3.Inject 50 µL into LC-MS system.

LC method

Mobile phase A: 0.1% formic acid in water Mobile phase B: 0.1% formic acid in methanolColumn: Thermo Scientific TM Hypersil GOLDM aQ 5µ 50x2.1mm

TABLE 1. HPLC Gradient Method

Mass Spectrometry Method

APCI ionization source

Data acquisition method: parallel reaction monitoring (PRM) experiment collecting MS2 spectra for each analyte.

Resolution: 17.5K

Data Analysis

Thermo Scientific™ TraceFinder 3.2 software was used for all dataprocessing and analysis.

Method Performance EvaluationQC samples were prepared by spiking previously analyzed donor plasmato concentrations specified in Table 2 and Figure 2.

TABLE 2. QC Samples Concentrations

ResultsFIGURE 1. 25OHD2, 25OHD3 MS/MS Spectrum

FIGURE 2. Chromatogram of QC Plasma Samples

QC1 QC2 QC3

25OHD2

25OHD3

6-25OHD3

(IS)

FIGURE 3. Calibration Curves with Lowest Calibration Standard Peaks

25OHD2

4.0 ng/mL

25OHD3

4.0 ng/mL

d6-25OHD3

(IS), 25 ng/mL

©2015 Thermo Fisher Scientific. All Rights Reserved.

All other trademarks are the property of Thermo Fisher Scientific and its subsidiaries.

This information is not intended to encourage use of these products in any manners that might infringe the intellectual property rights of others.

Evaluation of Bench-top Quadrupole Orbitrap Ultra High Resolution MS for Use in Clinical Research in Rapid Quantitative Analysis of Vitamin D in Human PlasmaMindy Gao, Marta KozakThermo Fisher Scientific, San Jose, CA, USA

For research use only. Not for use in diagnostic procedures.

Time (min) Flow rate (mL/min) %A (mobile phase)0 0.70 200.2 0.70 200.3 0.70 51.5 0.70 51.6 0.70 202.0 0.70 20

021715_APCI_4xP_D1_Cal_7 #787 RT: 1.17 AV: 1 NL: 3.64E6F: FTMS + c APCI corona Full ms2 395.33@hcd20.00 [50.00-420.00]

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83.0860229.1583119.0856

209.1322251.1792135.1168 159.1163 185.1320 307.2419

279.2106

335.2729

Water lost fragment

Quantifier

25OHD2

Quantifier

Water lost fragment

25OHD3

RT: 0.00 - 2.00 SM: 5B

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NL: 7.56E4m/z= 269.1848-269.1948 F:FTMS + c APCI corona Fullms2 395.33@hcd20.00 [50.00-420.00] MS021715_APCI_4xP_D1_PlasmaL_5

NL: 1.99E5m/z= 257.2214-257.2314 F:FTMS + c APCI corona Fullms2 383.33@hcd15.00 [50.00-410.00] MS021715_APCI_4xP_D1_PlasmaL_5

NL: 2.07E6m/z= 263.2588-263.2688 F:FTMS + c APCI corona Fullms2 389.37@hcd20.00 [50.00-415.00] MS021715_APCI_4xP_D1_PlasmaL_5

RT: 0.00 - 2.00 SM: 5B

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NL: 1.54E5m/z= 269.1848-269.1948 F:FTMS + c APCI corona Fullms2 395.33@hcd20.00 [50.00-420.00] MS021715_APCI_4xP_D1_PlasmaM_2

NL: 3.63E5m/z= 257.2214-257.2314 F:FTMS + c APCI corona Fullms2 383.33@hcd15.00 [50.00-410.00] MS021715_APCI_4xP_D1_PlasmaM_2

NL: 2.65E6m/z= 263.2588-263.2688 F:FTMS + c APCI corona Fullms2 389.37@hcd20.00 [50.00-415.00] MS021715_APCI_4xP_D1_PlasmaM_2

RT: 0.00 - 2.00 SM: 5B

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NL: 2.38E5m/z= 269.1848-269.1948 F:FTMS + c APCI corona Fullms2 395.33@hcd20.00 [50.00-420.00] MS021715_APCI_4xP_D1_PlasmaH_2

NL: 5.64E5m/z= 257.2214-257.2314 F:FTMS + c APCI corona Fullms2 383.33@hcd15.00 [50.00-410.00] MS021715_APCI_4xP_D1_PlasmaH_2

NL: 2.62E6m/z= 263.2588-263.2688 F:FTMS + c APCI corona Fullms2 389.37@hcd20.00 [50.00-415.00] MS021715_APCI_4xP_D1_PlasmaH_2

10.0 ng/mL 30.0 ng/mL20.0 ng/mL

Collision energy (20 eV) was optimized to maximize response of quantifying fragment ion (m/z=269.1893)

Collision energy (15 eV) was optimized to maximize response of quantifying fragment ion (m/z=257.2257)

25.1 ng/mL 39.9 ng/mL 60.8 ng/mL

4 ng/mL 4 ng/mL

Calculated Amt %Diff3.98 -0.4509.97 -0.28026.1 4.5050.1 0.12096.1 -3.88

Calculated Amt %Diff3.96 -1.1010.2 1.9526.3 5.0846.7 -6.58101 0.640

Analyte QC1 QC2 QC3%RSD

25-Hydroxyvitamin D2 6.30 - 12.7 5.33 - 13.0 2.77 - 5.3025-Hydroxyvitamin D3 3.21 - 7.64 2.64 - 5.89 3.70 - 4.70

%Recovery25-Hydroxyvitamin D2 87.0 - 100 99.9 - 109 102 - 10625-Hydroxyvitamin D3 82.9 - 83.5 94.5 - 96.3 91.1 - 101

* 5 replicates of QC samples containing 25OHD2 and 25OHD3 were proceed and analyzed in 3 batches

Analyte QC1 QC2 QC3%RSD

25-Hydroxyvitamin D2 10.5 9.01 4.5125-Hydroxyvitamin D3 5.56 3.93 6.1

%Recovery25-Hydroxyvitamin D2 93.2 105 10425-Hydroxyvitamin D3 82.9 95.1 97.3

* 5 replicates of QC samples containing 25OHD2 and 25OHD3 were proceed and analyzed in 3 batches

Compound Precursor (m/z)

Quantitation Fragment (m/z)

Collision Energy (V) Polarity

25OHD2 395.3308 269.1898 20 Positive25OHD3 383.3308 257.2264 15 PositiveD6-25OHD3 (IS) 389.3685 263.2638 20 Positive

Analyte Cal-4 Cal-10 Cal-25 Cal-50 Cal-100%RSD

25OHD2 1.60 2.52 4.27 1.65 2.7125OHD3 4.72 1.37 4.77 2.01 3.86

%Recovery25OHD2 99.7 101 96.8 105 96.925OHD3 100 101 97.0 98.8 103

* 5 replicate injections of each calibration standard containing 25OHD2 and 25OHD3 were performed to demonstrate the system reproducibility

Analyte Plasma-1 Plasma-2 Plasma-3 Plasma-4 Plasma-5%RSD

25OHD2 3.65 5.36 9.17 5.90 10.625OHD3 2.70 3.48 1.09 4.31 6.99

%Recovery 25OHD2 77.2** 91.7 79.9** 86.5 85.325OHD3 112 104 106 109 111

* 15 ng/mL of each analyte was spiked in 5 different plasma samples in 5 replicates

** 25OHD2 % recovery will be increased when deuterated analog will be used as internal standard.

FIGURE 4. Chromatogram of Lowest Calibration Standard

RT: 0.80 - 1.50 SM: 5B

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NL: 4.23E4m/z= 257.2251-257.2277 F:FTMS + c APCI corona Fullms2 383.33@hcd15.00 [50.00-410.00] MS021715_APCI_4xP_D1_Cal_3

NL: 2.24E6m/z= 263.2625-263.2651 F:FTMS + c APCI corona Fullms2 389.37@hcd20.00 [50.00-415.00] MS021715_APCI_4xP_D1_Cal_3

RT: 0.80 - 1.50 SM: 5B

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NL: 4.23E4m/z= 257.2251-257.2277 F:FTMS + c APCI corona Fullms2 383.33@hcd15.00 [50.00-410.00] MS021715_APCI_4xP_D1_Cal_3

NL: 2.24E6m/z= 263.2625-263.2651 F:FTMS + c APCI corona Fullms2 389.37@hcd20.00 [50.00-415.00] MS021715_APCI_4xP_D1_Cal_3

Chromatogram reconstructed with mass accuracy of 5 ppm

System reproducibility was evaluated by analyzing 5 replicates of eachcalibration standard (Table 6).

TABLE 3. PRM transitions of targets and internal standards

Method accuracy was evaluated by obtaining %recovery for NIST controls.

Method precision was evaluated by analyzing 5 replicates of each QC sample in 3 different days (Table 4, Table 5).

Matrix effects were evaluated by spiking previously analyzed plasma from 5 different donors with 25OHD3 and 25OHD2 concentrations of 15 ng/mLand calculating % RSD and % recovery from 5 replicate analysis (Table 7).

Analyte/Concentrationng/mL QC1 QC2 QC3

25-Hydroxyvitamin D2 10.0 20.0 30.025-Hydroxyvitamin D3 25.1 39.9 60.8

TABLE 7. Matrix Effects *

TABLE 6. System Reproducibility *

TABLE 5. Inter-assay Precision and Accuracy *