dna image cytometric measurement as a surrogate end point ... · vol. 6, 849-855, october 1997...
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Vol. 6, 849-855, October 1997 Cancer Epidemiology, Biomarkers & Prevention 849
DNA Image Cytometric Measurement as a Surrogate End Point
Biomarker in a Phase I Trial of a-Difluoromethylornithine
for Cervical Intraepithelial I
Iouri V. Boiko, Michele Follen Mitchell,2Dibip K. Pandey, R. Allen White, Wei Hu,Anais Malpica,3 Kenji Nishioka,4 Charles W. Boone,E. Neeby Atkinson, and Walter N. Hittelman
Departments of Clinical Investigation (I. V. B.. W. H., W. N. H.], Gynecologic
Oncology [M. F. M., D. K. P.], Biomathematics [R. A. W., E. N. Al, Pathology
IA. M.], and Surgical Oncology [K. NI, The University of Texas M. D.Anderson Cancer Center. Houston, Texas, 77030; and Chemoprevention
Branch, National Cancer Institute, Division of Cancer Prevention and Control.
Bethesda, Maryland 20892 [C. W. B.l
Abstract
Cervical intraepithelial neoplasia grade 3 (CIN 3) isconsidered a high-risk precursor of invasive cervicalcancer. a-Difluoromethybornithine (DFMO) is apromising antiproliferative chemopreventive agent. Thepurpose of this study was to evaluate image cytometricmeasurement of nuclear DNA (1CM-DNA) as a surrogateend point biomarker (SEB) in a Phase I trial of DFMOfor CIN. Thirty patients with CIN 3 were treated withDFMO at five doses, ranging from 0.0625 to 1.0 g/m2/day,for 1 month. Half of the patients had histologicalresponses. Twenty-five pre- and posttreatment cervicalbiopsy specimens (from 11 responders and 14nonresponders) were available for this analysis. 1CM-DNA was performed on 4-�.tm sections cut from formalin-fixed tissue blocks and stained with a thionin-S02Feulgen reaction. ICM-DNAs for each case wereexpressed as normalized measurements (against thenuclear modal absorbance of lymphocytes) of theabsorbance of each cell of interest and were presented inbar histograms. The mean normalized summedabsorbance (�ODn) was obtained as a mean histogram ofthe cell population of interest. Nineteen (76%) of 25
patients had a significant decrease in �OD� after DFMOtreatment. Posttreatment values were significantly bower
than pretreatment values in a paired analysis, andresponders had significantly lower values thannonresponders. Analyses of different 1CM-DNA
Received 12/10/96; accepted 6/27/97.
The costs of publication of this article were defrayed in part by the payment of
page charges. This article must therefore be hereby marked advertisement in
accordance with I 8 U.S.C. Section 1734 solely to indicate this fact.
‘ This work was supported by National Cancer Institute Contract CN-25433-02.
2 To whom requests for reprints should be addressed, at Department of Gyneco-
logic Oncology, Box 67, The University ofTexas M. D. Anderson Cancer Center,
1515 Holcombe Boulevard, Houston. TX 77030. Phone: (713) 745-2564: Fax:(713) 792-7586.
3 Present address: Brown and Associates Medical Laboratories. 8076 Del Rio.
Houston. TX 77054.
4 Present address: 7820 Kendalla Drive, Houston, TX 77036.
references, including percentile values of �OD�distribution, DNA malignancy grade, and 5c exceedingrate, showed a decrease of mean �OD� during DFMOtreatment. In addition, the summed posttreatment �OD�histograms also showed progressively shorter rightshoulders compared with pretreatment histograms inboth responders and nonresponders. We concluded that
the modulation of �OD� reflected the chemopreventioneffect of DFMO even before morphological changesappeared, and thus, 1CM-DNA may be useful as a SEB inchemoprevention trials of DFMO. Additional reasons forusing 1CM-DNA as a SEB are the relative simplicity ofits use, the high accuracy of the results, the low cost of
the reagents, the ability to use small tissue samples, andthe objectivity and reproducibility of the procedure.
Introduction
Cervical cancer remains an important health problem; it is thesecond most common cancer in women worldwide ( I ). CIN 3,�
which includes severe dysplasia and carcinoma in situ. is ahigh-risk precursor of invasive cervical cancer and is thus
suitable for the study of chemoprevention of cancer (2, 3). Onechemopreventive agent that is promising in the cervix is
DFMO, a potent antiproliferative agent that was used in a PhaseI chemoprevention trial in CIN 3 (3). DFMO will soon be testedin a Phase II placebo-controlled trial in CIN.
DFMO, a specific inhibitor of ornithine decarboxylase,inhibits polyamine synthesis. Despite extensive research ef-forts, the precise function of polyamines in cellular physiology
is not yet well understood. Basic pobyamines are capable ofnoncovalent interactions with nucleic acids and proteins (4-6),and these interactions may stabilize DNA structure and protect
DNA from nuclease digestion (5, 7), alter sequence-specificDNA-protein interactions, change the regulatory process in the
chromatin of nuclei (8, 9), and affect the attachment of DNA to
the nuclear matrix, possibly affecting replication and transcrip-
tion (5, 10, Il). Because DFMO inhibits ornithine decarboxy-base activity and pobyamine synthesis, it can inhibit or delayDNA synthesis both in vitro and in vivo ( 1 2, 1 3). This processhas been associated with decreased cell proliferation (12, 14),loss of the mitogenic response to growth factor stimulation( I 5), and reduction of proto-oncogene (c-fos and c-tnvc) ex-
pression (16).Here, we investigated two hypotheses. The first was that
DFMO decreases DNA synthesis or total DNA content in CIN
S The abbreviations used are: CIN 3, cervical intraepithelial neoplasia grade 3;
DFMO. a-difluoromethylomithine: SEB. surrogate end point biomarker: 1CM-
DNA, image cytometric measurement of nuclear DNA: � normalized
summed absorbance: DNA-MG, DNA malignancy grade: 5cER. Sc exceeding
rate: df, degrees of freedom.
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850 DNA Image Cytometry in a Cervix Chemoprevention Trial
3 lesions. The second involved a potential SEB for evaluatingthe effects of DFMO.
The end point of interest in chemoprevention studies iscancer incidence reduction ( I 7). However, this end point re-
quires years of follow-up, and such studies are expensive. SEBsare intermediate markers of carcinogenesis that allow trials to
be of shorter duration, to require fewer subjects, to be lower in
cost, to use small tissue samples, and to aid in beaming moreabout the carcinogenic process ( I 7).
For several decades, flow cytometric measurement of nu-clear DNA and 1CM-DNA have been used for research and
diagnostic purposes as biomarkers of proliferation and neopbas-tic transformation (1 8-24). For example, an increase in nuclearDNA during the progression of CIN lesions has been shown
(21 , 22). 1CM-DNA has also been used for monitoring doseeffectiveness in some chemotherapeutic studies (23, 24).
Recently, 1CM-DNA has been proposed for purposes ofSEB development because it uses an intact tissue sample, and
thus, important information about tissue architecture and thedegree of neoplastic progression is retained (17). Despite rel-
ative limitations of 1CM-DNA in tissue sections (25, 26), well-standardized analysis (27) of nuclear summed absorbance canstill reflect the relative total amount of cell DNA. Thus, oursecond hypothesis was that DFMO decreases DNA synthesisand/or total DNA content in CIN 3 lesions and that 1CM-DNA
measures that reflect DFMO’s effect on DNA content mayserve as SEBs of the effects of chemoprevention. To test ourhypotheses, we used 1CM-DNA to examine pre- and posttreat-ment biopsies from a group of CIN 3 patients during a chemo-prevention trial of DFMO.
Materials and Methods
Patient Groups and Tissue Sampling. Thirty patients with
CIN 3 involving over one-third of the surface area of the cervix(i.e., areas - I .0-1 .5 cm in diameter) were treated in a Phase I
chemoprevention trial. Six patients were assigned to each offive dose levels of DFMO, ranging from 0.0625 to 1.0 g/m2/day, for I month. Pretreatment colposcopicalby directed biopsysamples (measuring 1 X 2 X 2 mm) were compared with
posttreatment colposcopicalby directed cone biopsy samples(measuring 3 cm in diameter at the cone base and 2 cm inheight). Fifteen (50%) of these patients had histological re-sponses after treatment, of which 5 were classified as complete
responses (a posttreatment diagnosis of metaplasia or reactiveand granulation tissue) and 10 were evaluated as partial re-sponses [CIN lesions of bower grade (i.e. , 1 or 2) than before
treatmentj. Samples from 25 of the 30 patients were availablefor 1CM-DNA analysis because of biopsy size and the need foradequate field size.
Preparation of Materials. The tissue blocks were randomlyordered, and the same microtome was used to cut all of thespecimens at the same time. Serial 4-tam-thick tissue sectionswere stained with H&E for light microscopic evaluation, andother sections were stained for the Feulgen reaction using theprotocol of Xibbix Technologies (Vancouver, British Columbia,
Canada; Ref. 28). All slides were stained at the same time,under the same conditions. To increase the accuracy of thisstudy, paired pre- and posttreatment samples from each patientwere cut and treated under the same conditions, at the same
time. Briefly, following deparaffinization, the samples wererehydrated and postfixed in Boehm-Sprenger fixative. After 45
mm of acid hydrolysis (5 N HCI; 23#{176}C),the sections werestained with thionin-SO2, washed, dehydrated, cleared in xy-lene, and mounted for image analysis. The pre- and posttreat-
ment H&E-stained slides were reviewed to identify the patho-logical areas of interest, including dysplastic and reactive areas
in the epithelium, by two pathologists (A. M. and I. V. B.) and
used as templates to map Feulgen-stained slides.
Image Analysis. At The University of Texas M. D. Anderson
Cancer Center (Houston, TX), the CytoSavant computer-
assisted image analysis system (Oncometrics Imaging Co.,
Vancouver, British Columbia, Canada) was used for 1CM-DNA
analysis (29). This system has a scientific-grade charge-coupled
device, which is able to give a small pixel size, 100% fill factor,high quantum efficiency, low readout noise, wide dynamic
range, good linearity, and geometric stability (Xillix Technol-ogies). The charge-coupled device transducer is positioned in
the primary image plane of a Nikon 20/0.75 Plan Apo objective.
This arrangement results in the acquisition of a chromatically
and geometrically correct image with square pixels. On aver-
age, each nucleus is covered by over 500 pixels. The device
uses algorithms for the automated detection of the nuclearboundaries along the highest local gradient between the nuclear
stain and unstained cytoplasmic background, which defines the
nuclear boundary in a precise, objective, and reproducible way.
Cell Selection. Lymphocytes were used as internal standardcontrols to normalize each slide and to correct for staining
variations. From each tissue section, nuclear images of 50 ± 15
(mean ± SD) lymphocytes and 130 ± 40 epithelial nuclei frompreviously mapped CIN 3 areas were collected by a pathologist
(I. V. B.) in a semi-interactive procedure and stored in thecomputer memory. The collection of nuclei in interactive mode
helped to control selection bias (only nonoverlapping nuclei
with easily detected boundaries and without “capping” were
chosen). Additional control of cell quality was performed byexamination of a computer-stored cell gallery, which allowed a
magnified display of the stored image of each nucleus. In this
way, the scored cells could be reviewed, and fragmented cellswere eliminated from the analysis. The number of selected
nuclei depended on how much of the pathological area of
interest was on the analyzed slide. The coefficient of variation
of �OD of lymphocytes was 5%.
Epithelial cells (about 100 per sample) from normal-ap-
pearing regions that were adjacent to CIN lesions were also
analyzed in available samples to determine the mean �OD ofnormal epithelial cells in relation to the modal �OD of lym-
phocytes. A correction factor of 1 . 1 5 was used to account for
the down-shift in the �OD distribution due to the difference inchromatin compaction in lymphocytes and epithelial cells. Af-
ter the correction factor was applied, the modal �OD of lym-
phocytes was summed as a normalized unit of measurement
(which corresponded to the unit “2c,” which has been used in
previous studies) and linearly extended to establish the normal-
ized �OD scale.
Interpretation of DNA Histograms. ICM-DNAs for eachcase were expressed as normalized measurements (against thenuclear modal absorbance of lymphocytes) of the �OD of each
cell of interest and were presented in bar histograms. The
following data were obtained and used as 1CM-DNA refer-
ences: (a) �ODn for each case, obtained as a mean �ODn
histogram of the cell population of interest (30); (b) DNA-MG,
based on the “2c deviation index” and presented as a continuousscale ranging from 0.01 to 3.0 (3 1 ); (c) 5cER, defined as the
percentage of cells having a “DNA content” of more than Sc
(32); and (d) percentile value of �ODn distribution, defined asrates of �ODn at the 5th, 25th, 50th, 75th, and 95th percentile
points of the �OD� histogram.
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Cancer Epidemiology. Biomarkers & Prevention 851
Statistical Analysis. A nonparametric (Wilcoxon) test of sig-nificance was performed to assess the differences between
�ODn in pre- and post-DFMO treatment CIN 3 samples. The
SPSS statistical software was used for analysis.The modulation of �ODn during DFMO treatment was
analyzed also using a mixed effect linear model. Specifically,we assumed
Yjko+�tXt+13�2+13�X3+1.Li+Y�,+#{128},jk,
where: (a) Y�3k �5 the logarithm of the �OD� for patient i, group
j, and replication k; (b) group 1 is composed of pretreatmentsamples from nonresponders; group 2 is composed of pretreat-ment samples from responders; group 3 is composed of post-
treatment samples from nonresponders; and group 4 is com-posed of posttreatment samples from responders; (c) x1 is 0 for
pretreatment data and 1 for posttreatment data; (d) x2 is 0 for
data from nonresponders and 1 for responders; (e) �. whichrepresents the random effect for patient i, is normally distrib-uted with mean 0 and variance o�2; (j) �y which represents therandom effect of groupj within patient i, is normally distributedwith mean 0 and variance a’,2; and (g) �.jk is normally distrib-
uted with mean 0 and variance o�.Thus, the patient is considered a random factor, response/
nonresponse is a between-patient factor with both fixed andrandom components, and pretreatment/posttreatment is a with-in-patient factor with both fixed and random components. The
design is unbalanced with unequal replicates. The variance ofcase means around the group mean is permitted to differ amongthe four groups. The model was fit using the lme function of
S-PLUS, version 3.4. All significanttests were performed using
the likelihood ratio test.
Results
Data for patient ages, doses of DFMO, �OD� of pre- andposttreatment samples, and histological response are presentedin Table 1 . The mean age was the same (29 years) in responders
and nonresponders. Nineteen (76%) of the 25 patients studiedshowed a decrease in �ODn after DFMO treatment. Threepatients had no �ODn changes, and three showed an increase of
�ODn after treatment. Although no significant dose-dependentresponse in �ODn was detected as a fraction of dose, perhaps
due to the small number of cases, all patients who had increasesof �ODn following treatment had received bow (0.062�-0.12S
g/m2/day) doses of DFMO.According to histological diagnosis, there were 1 1 re-
sponders and 14 nonresponders among the 25 patients who hadevaluabbe pre- and posttreatment samples available for the
study. Only 1 of 1 1 responders had no �OD� change afterDFMO treatment (all other responders had decreases in �ODn
5 of 14 nonresponders had either no change or an increase inposttreatment �ODn).
The group mean values of �OD� according to histologicalresponse and treatment category are shown in Table 2. There
was a trend for lower pretreatment �ODn in responders than innonresponders; however, this trend was not significant. Al-
though both the responders and nonresponders showed an over-
all significant decrease in �ODn after DFMO treatment, theresponders’ values dropped more than the nonresponders’ val-ues, which resulted in a significant difference between �ODn
values for responders and nonresponders in posttreatment sam-pies ( I .25 versus 1 .5, respectively).
The values obtained from DNA-MG analysis are pre-sented in Table 3. DNA-MG, which is based on a 2c deviationindex distribution, is defined as the sum of the squares of the
Table I Distribution of age, pre- and posttreatment �OD� and histologicalresponse by DFMO dose level
Dose level Age (�OD�) Histological
response(g/m2/day) (yr) Pretreatment Posttreatment
1.00 41 1.19 1.03 PR”
30 1.72 1.05 PR
23 1.51 1.38 NR
24 1.53 1.42 NR
35 1.94 1.85 NR
0.50 27 1.27 1.16 PR
40 2.11 1.41 NR
28 2.01 1.19 NR
20 1.34 1.31 NR
0.25 23 1.19 1.18 PR
29 1.48 1.11 CR
29 1.63 1.26 NR
25 1.60 1.28 NR
0.125 39 1.75 1.81 NR
31 1.30 1.55 NR
40 1.75 1.11 PR
25 2.21 1.14 CR
26 1.37 1.07 CR
22 1.33 1.19 PR
0.06 22 1.69 1.33 NR
23 1.38 1.41 NR
36 1.88 1.76 NR
26 1.43 1.51 NR
22 1.46 1.13 CR
40 1.30 1.20 CR
Mean ± SE 1 .58 ± 0.06” 1 .3 1 ± 0.05”
“ PR, partial response; NR, no response; CR, complete response.
“P < 0.01.
Table 2 Mean 10 D� by DFM 0 treatment and h istological respon. cc category
Histologicalresponse
No. ofPatients
Mean
(�OD,)
pretreatment
Mean
(�OD�)
posttreatment
Nonresponders 14 1.79 1.50 0.04
Responders 10 1.69 1.25 <0.01
P 0.52 0.02
Table 3 DNA-MG values by DFMO treatment and histologi cal response
category
Histological
response
DNA-MG P
Pretreatment Posttreatment
Responders 2.50 2.05 <0.01
Nonresponders 2.63 2.43 0.04
Total 2.58 2.26 <0.01
differences between the �OD� of single cells and the 2c value,divided by the number of measured cells (31, 32). In our study,2c was evaluated as the modal �OD of lymphocytes multiplied
by a correction factor. Mean DNA-MG in this study was
significantly lower in posttreatment than in pretreatment sam-pies for both responders (P < 0.01 ) and nonresponders (P <
0.04).Values for 5cER, the number of cells with �ODn exceed-
ing Sc, were also lower in posttreatment samples than in pre-treatment samples (Table 4). There was a posttreatment de-crease in both responders and nonresponders.
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852 DNA Image Cytometry in a Cervix Chemoprevention Trial
Table 4 SeER by DFMO treatment and histological response category
Histological
response
No. of
pattents
No. of patients with SeER Cells Mean 5 cER (%)
Pretreatment Posttreatment Pretreatment Posttreatment
Nonresponders I I 9 2 5.5 0.3 0.03
Responders 14 13 9 9.4 4.6 0.05
Total 25 22 11 8.3 3.1 0.01
Table 5 Percentile values of �OD,, distribution by DFMO treatm
histological response category
ent and
Treatment and Percentile of �OD�
histological response 5th 25th Sorb 75th 95th
Responders
Pretreatment 0.96 1.25 1.49 2.01 2.92
Posttreatment 0.80 1 .03 1.21 1.40 1.82
Nonresponders
Pretreatment 0.97 1.29 1.62 2.16 3.04
Posttreatment 0.80 1.13 1.37 1.76 2.64
Post/Pretreatment ratio
Nonresponders t).83 0.88 0.85 0.81 0.87
Responders 0.83 0.82 0.81 0.70 0.62
After DFMO treatment, both responders and nonre-sponders had a left shift in summed posttreatment �ODn his-
tograms compared with pretreatment histograms. However, therates of this shift were different and resulted in a prominent
shape difference between the posttreatment �ODn histogramsof responders and nonresponders. This difference can be ex-
plained by changes in individual �OD� histograms after DFMOtreatment. Ten of 1 1 responders but only 9 of 14 nonrespondershad a posttreatment decrease of � So, the summed post-treatment �OD� histogram of nonresponders included two
components. one incorporating histograms of patients who hada decrease (as did almost all of the responders) and one incor-porating histograms of patients who had no change or an
increase. The 5th, 25th, 50th, 75th, and 95th percentile points of
the �ODn distribution histograms give a quantitative descrip-tion of the data presented in the �ODn histograms (Table 5).
To show that the distribution of slide thickness was ran-dom and did not affect �ODn measurements, we checked area
size and �OD of lymphocytes in pre- and posttreatment sam-pIes. The chromatin structure features of lymphocytes were also
compared to prove that DFMO did not affect chromatin struc-ture and that �ODn changes were, therefore, not an aftereffectof acid hydrolysis from the Feulgen reaction. The data for meanarea, SOD, and chromatin structure of pre- and posttreatment
lymphocytes show there was no significant DFMO effect on
any feature in the lymphocytes (Table 6).Additional information about the relationship between in-
dividual �ODn value distribution within and between differentgroups of patients before and after DFMO treatment was ob-tamed by carrying out a mixed-effect linear model analysis. Thevariances of groups 1 , 2, and 3 did not differ significantly (f= 0.336, df = 2, P = 0.85); however, the variance of group 4(posttreatment, responders) was significantly different from theremaining variances (� = 18.610, df 3, P < 0.001). Theinteraction between treatment and response was not significant
Uv�t 1 .094, df = I , P = 0.30), but treatment and responsewere individually significant (treatment, � = 19.828, df 1,
P < 0.001; response. � = 7.726, df = I, P = 0.005). Esti-mated values are: f3� - 0.5447, f3� = -0.2293, �2 = -0.12 19,
Table 6 Mean area, IOD,. and chromatin structure values of lymphocytes inpretreatment and posttreatment samples
Area IOD,, Entropy Energy Correlation Contrast
Pretreatment 199 91.7 3.2096 0.073 220.6 56
Posttreatment 205 92 3.2088 0.073 2 17.7
P 0.10 0.78 0.88 1 0.37 0.41
o’i = #{176}‘2= O�3 = 0.1816, O�4 = 0.0298, o’,� 0.0035, and o� =
0.2987. Thus, posttreatment values were bower than pretreat-
ment values, and responders had lower values than did nonre-sponders. These results of the mixed modal analysis support thehypothesis that DFMO significantly affected the �
Fig. I shows the individual �OD� histograms for biopsy
specimens from three patients: a nonresponder, a partial re-sponder, and a complete responder. These histograms demon-strate a shift in the DNA index for the patients who responded
and no shift for the patients who did not respond.
For each patient, two histograms were constructed, one forpretreatment �ODn and one for posttreatment �ODn. The his-
tograms represented the proportion of cells falling in a bin,based on rank percentile of optical densities. The individual
histograms were then averaged, giving them equal weight, toget the composite histogram. A composite histogram of eachgroup was then created by averaging the groups’ individualhistograms, thus giving equal weight to each case.
As shown in Fig. 2, the pretreatment biopsies from re-sponders and nonresponders showed similar �OD� distribu-
tions; however, there was a tendency toward a more normalizedpattern in the responders. Following treatment, there was a leftshift in distribution for both responders and nonresponders.
Discussion
CIN 3 is considered a high-risk precursor to invasive cervicalcancer (2, 3). Both genomic instability and proliferative dys-regulation play important roles in the progression of CIN 3lesions and could result in increased mean DNA content (17).Cells with high DNA content have been found to have a
particular proliferative behavior and could play an importantrole in tumor evolution (33) and in the progression of CIN 3 to
invasive cervical carcinoma. It has been shown that “high-risk”CIN 3 lesions, those lesions residing beside invasive cancers,
have a higher percentage of cells with high DNA content thando CIN 3 lesions that are not associated with cancer (22).Therefore, the opposite process, decreasing the number of cellswith high DNA content in CIN 3, may reflect an abolition of
“malignant” behavior of CIN 3 and a reversal of precancerouslesions.
The “slicing problem” makes the precise determination ofDNA content and modal stem-line ploidy difficult on tissue
sections (25, 26). The method of correcting DNA pboidy meas-urements in tissue sections (25) can be used to address thisproblem only for special cell populations with “spherical nucleiand uniform DNA concentration throughout the nucleus.”
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8
A
N
0
fC
eIIS
B
N
0
fC
C
IIS
1.00 1.00 2.00
EOD�
3.00 4.00
11
Na
0
I �.
C
C
l
S 2�
0
EOD�
I0.00
Ii.#{243}o 2.#{243}o
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Cancer Epidemiology, Biomarkers & Prevention 853
C
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e1
IS
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eIIS
Ill L�I�2.00 3.� 4.00
�oDn
Fig. 1. Individual �OD, histograms from three CIN 3 patients before and after DFMO treatment by histological response. A. a nonresponsive patient: B, a partially
responsive patient: C, a complete responsive patient.
Because the CIN 3 cell populations in our study were quite
heterogenic, we did not use this method. However, we believethat the slicing problem did not affect our data, because we
measured �OD� in pairs: pre- and posttreatment samples from
each patient. Under these conditions, paired comparison was
achieved in genetically similar (especially for nonresponders)cell populations before and after DFMO treatment. Uniformconditions of slide preparation and measurement of pre- and
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0.1
%
0
I
A0.1
04
. 08
.02
. 06
B
0
I
C
e
IS
.04
I
0.1
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I
EOD� EOD�
2
C D0.1
0 .08
I
.06
C
e
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S
.04
I 2 3 4
�OD�
Fig. 2. The summed pre- and posttreatment �OD,, histograms for responders (A and B) and nonresponders (C and D).
854 DNA ImageCytometry in a Cervix Chemoprevention Trial
C
e
IS
C
C.
S
posttreatment lymphocytes were used as controls to demon-strate that no factors other than DFMO affected � Underthese circumstances, we believe that �OD� changes reflect amodulation of DNA content during DFMO treatment.
Our data show that all patients with CIN 3 lesions had highlevels of � and nonresponders showed a trend to havemore high pretreatment �OD� than responders. These datamean that both responders and, especially, nonresponders had
in pretreatment samples high numbers of cells with high DNA
content that contribute to the malignant behavior of CIN 3 (22).
After I month of DFMO administration, reduction of
�ODn was achieved in 10 of 1 1 responders and in 9 of 14nonresponders. If a posttreatment �ODn decrease in responderscan be associated with a change in the histological grade of CINlesions (21 , 22), the reduction of �OD� in nonresponders sug-
gests that DFMO could decrease “DNA amount” in CIN 3lesions even before the appearance of morphological changes.Whether this change is due to a decrease in proliferation or
elimination of particular clones is unknown. We believe thatthese results suggest antiproliferative activity of DFMO be-
cause, as was shown in an animal model, DFMO can inhibit ordelay DNA synthesis and decrease proliferation (12-14). These
data agree with our findings that DFMO can decrease the level
of cell proliferation, which has been detected by proliferating
cell nuclear antigen and MPM-2 modulation (34, 35).To study the antiprobiferative activity of DFMO, we ana-
lyzed the �ODn histograms with different descriptors. The
visual left shift of posttreatment �ODn histograms, which was
quantitatively detected by analysis of percentile values of
�ODn distributions and a decrease of DNA-MG and ScER,
shows a depletion in cell number and in the right shoulder of the
histogram. These changes probably correspond to depletion in
cells in the S-phase and G,-M of the cell cycle. These data
suggest that DFMO has an antiprobiferative and cytostatic ef-
fect. The evidence that DFMO did not affect �OD in lympho-
cytes also confirms the cytostatic, rather than cytotoxic, effect
of DFMO; it selectively affected DNA content in the probifer-
ative cell population (CIN 3) but not the quiescent one (lym-
phocytes).To be sure that this result was not dependent on the quality
of the image analysis system or on the operator, additional
measurements of �OD� in the same samples were performed in
the Cancer Imaging Department of the British Columbia Cancer
Agency (Vancouver, British Columbia, Canada) on their
CytoSavant system by another operator. This independent study
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Cancer Epidemiology, Biomarkers & Prevention 855
also detected a significantly lower �OD� after DFMO treatmentthan that in pretreatment samples (data not shown).
In conclusion, our study suggests that: (a) the �OD� in
CIN 3 tissues significantly decreased during the DFMO che-moprevention trial, and this decrease was due to a depletion of
cells with high DNA content; and (b) the modulation of �ODn
reflected the chemoprevention effect of DFMO before the ap-
pearance of morphological changes, providing a rationale forthe possible use of 1CM-DNA as a SEB in chemopreventiontrials with DFMO. Additional reasons for using 1CM-DNA as
a SEB are its relative simplicity, low cost of reagents, ability to
use small tissue samples, objectivity, and reproducibility.
Acknowledgments
We are grateful for helpful comments from Branko Palcic, Ph.D., Calum
MacAuley, Ph.D., and James Bacus, Ph.D. Editorial assistance from Sunita
Patterson and manuscript preparation by Pat Williams are appreciated.
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on February 26, 2021. © 1997 American Association for Cancer Research. cebp.aacrjournals.org Downloaded from
1997;6:849-855. Cancer Epidemiol Biomarkers Prev I V Boiko, M F Mitchell, D K Pandey, et al. cervical intraepithelial neoplasia.biomarker in a phase I trial of alpha-difluoromethylornithine for DNA image cytometric measurement as a surrogate end point
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