bioinformatics lab tuesday, march 9, 2010 kristoffer chin salomon garcia michael pi ñ a
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Recurring conformation of the human immunodeficiency virus type 1 gp120 V3 loop. Stanfield RL, Ghiara JB, Ollmann Saphire E, Profy AT, and Wilson IA. Virology (2003) Oct 10; 315(1) 159-73. BioInformatics Lab Tuesday, March 9, 2010 Kristoffer Chin Salomon Garcia Michael Pi ñ a. Outline. - PowerPoint PPT PresentationTRANSCRIPT
Recurring conformation of the human immunodeficiency virus type 1 gp120 V3
loop. Stanfield RL, Ghiara JB, Ollmann Saphire E, Profy AT, and
Wilson IA. Virology (2003) Oct 10; 315(1) 159-73
BioInformatics LabTuesday, March 9, 2010
Kristoffer ChinSalomon Garcia
Michael Piña
Outline
• Introduction– Background on HIV Structure– Background on HIV V3 Region
• Materials and Methods– Crystallography
• Results and Discussion• References
HIV has an outer surface of Glycoproteins
• gp120 responsible for binding to CD4 receptors and coreceptors, CCR5 or CXCR4
• gp41 anchors gp120 to the viral membrane providing noncovalent association
http://www.bijvoet-center.nl/cpc/research/HIVEnv/Env.jpg
Glycoproteins binding to CD4 T-cells
http://www.dkfz.de/de/f020/images/bosch/web_fig_1.jpg
V3 Region as part of gp120
• V3 important to viral infectivity• Progresses initial infection to AIDS
http://www.prn.org/images/uploads/86_tsibris_athe_fig2_680.gif
Introduction to the Stanfield et al. (2003) Study
• V3 regions have high propensity to elicit neutralizing antibodies
• V3 region inaccessible due to carbohydrates masking or tertiary or quaternary interactions with gp120 complex
• Is there a limited range of conformational states that gp120 can adopt?
• How is V3 loop recognized by antibodies and how an alteration of sequence, conformation, or exposure can affect it
Finding a dominant conformation for V3
• Fabs are antibodies that bind to V3 conformation• Fab 83.1, 50.1, and 59.1 bind to a similar
conformation of V3 region• NMR studies have shown V3 to form similar hairpin
loops• Stabilization of V3 loops to prevent change of
conformation through turns• 5 antibodies used for neutralizing and stablization
Materials and Methods
• Mab 83.1 was made by immunization of an ASW mice with cyclic peptide RP70
• Antibody was produced in ascites fluid of a mice and purified with an immobilized protein A column
• Fab was made from immunoglobin by cleavage
• Fab was concentrated to 15.0 mg/ml for crystallization studies
Fab Purification
• Fab was mixed with 16-mer peptide MP1 in a 6:1 mole ration
• Crystals were grown using sitting-drop vapor diffusion method with a reservoir solution of 1.6 M Na/K phosphate, 5% isopropanol, pH 6.0.
• Crystals grow as clusters of thin plates• Crystals used for this experiments grew over a
2-week period
Fab Crystallization procedure
• Crystals were cryocooled to liquid nitrogen temperatures in order to collect the data in a rapid manner
• The crystals were protected by putting them in a solution containing the following 25% glycerol, 1.6 M Na/K phosphate, 5% isopropanol, pH 6.0
• HKL2000 was used to format all of the data that was obtained
Structure determination
• Matthew coefficient was obtained by two Fab molecules
• Model was constructed from the constant region of Fab 58.2
• EPMR program was used to position the model in the cell
• EPMR also used to locate the first Fab molecule in the asymetric unit
Stanfield et al. 2003.
Model building and refinement
• TOM/FRODO was used to rebuild the mutated hybrid model and to correct the sequence and were subsequently refined with CNS version 1.1
• Refinement was carried with tight NCS restraints in the beginning and progressively released towards the end of refinement
Structural Analysis
• Kabat convention was used to number the molecules – Light and heavy chains are labeled using “L” and “H”– Peptide labeled “P” and was numbered according to
HXB2 isolate sequence
• HBPLUS was used to evaluate the Hydrogen bonds
• Contacsym program was used to assign van der waals contacts
Results and Discussion
• Rcryst and Rfree values were slightly higher than other structures determined at 2.6Å resolution
• Electron density maps were good quality • However, repeated refinement and manual
rebuilding of the structures caused the higher R-values
• Rcryst 28.8%, Rfree 32.6%• An index (0.45*l) close to an integer value is strong,
whereas close to one-half integer is weak
Stanfield et al. 2003.
Figure 1: comparison of V3 peptide conformations determined by X-Ray crystallography and NMR
Stanfield et al. 2003.
Figure 2: stereoview of electron density for the V3 peptide bound to Fab 83.1
Stanfield et al. 2003.
All CDR loops fall into their expected canonical classes with the exception of L1
• The L1 CDR loops have a 5 amino acid insertion after residue L27
• In both Fabs, the tip of this loop bends away from the antigen binding site in an unusual manner
• Comparison with other L1 loops shows the angle is about 9Å
Figure 3: the structure of the Fab 83.1-V3 peptide complex
Stanfield et al. 2003.
Figure 4: Noncanonical loops from Fab 83.1
Stanfield et al. 2003.
CDR H3 has a “kinked” base
• This was not predicted from its sequence• At least two other Fabs have kinked H3 bases
that were not predicted• AspH101 normally forms a salt bridge (with
Arg or Lys), but in this case it does not which is unexpected
Stanfield et al. 2003.
Figure 5: stereoview of H3 loop conformations from Fabs 83.1, B02C11, and 26-10
Stanfield et al. 2003.
The peptide makes contact with both the light and heavy chains from the Fab
• 110 total contacts for 1 molecule• 7 are hydrogen bonds with no charge-charge
interactions• 6 hydrogen bonds are to peptide main-chain
atoms• 1 bond to Arg side chain• The H3 CDR makes the most contacts
Stanfield et al. 2003.
The 83.1 peptide structure is the 4th crystal structure determined for a neutralizing antibody V3 peptide
complex
• Analysis of the 4 peptide reveals that 3 are very similar
• The 4th differs around the V3 region• The 4 antibody peptides were generated from
related mice• The antibodies themselves do not have structural
homology• The similarity among the conformation of the
peptides is not due to the similarity of the Fabs
Figure 6: comparison of the V3 peptide conformations
Stanfield et al. 2003.
Figure 7: the antibody combining site of Fab 83.1
Stanfield et al. 2003.
Figure 8: antigen binding sites of Fabs 83.1, 59.1, 58.2, & 50.1
Stanfield et al. 2003.
The peptides, although adopting the same shapes, bind in different orientations and locations in the
antibody
• The antibodies were chosen for ability to neutralize (bind to intact viruses)
• These peptide conformations should reflect “preferred” conformations of the V3 loop
• The identified V3 structures represent a recurring conformer on the intact virus
The X-rays of V3 peptides in complex with antibodies help define the range of V3
conformation• Studies suggest that V3 interacts with
coreceptors CCR5 and CXCR4 during cell entry• This information may be useful in the design
of V3 based inhibitors• Ultimately, a better understanding of the
gp120/gp41 structure (and the V3 region) is vital for understanding how HIV-1 carries out its binding and fusion activities
References• Stanfield et al. Recurring conformation of the human immunodeficiency
virus type 1 gp120 V3 loop. Virology (2003) Oct 10; 315(1) 159-73• http://www.bijvoet-center.nl/cpc/research/HIVEnv/Env.jpg• http://www.dkfz.de/de/f020/images/bosch/web_fig_1.jpg• http://www.prn.org/images/uploads/86_tsibris_athe_fig2_680.gif