Experiences from the Structure Determination of Human Cytomegalovirus Protease

Tong, Liang; Qian, Chungeng; Davidson, W.; Massariol, Marie-Josée; Bonneau, Pierre; Cordingley, Michael G.; Lagacé, Lisette

doi:10.1107/s0907444997006823

Cited by 8 publications

(5 citation statements)

References 16 publications

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“…The cause of this change in the dimer organization is currently unknown. Treatment of free enzyme crystals with Na 2 SO 4 also produced a re-organization of the dimer (and a significant improvement in diffraction quality) 3,11 . It appears that the herpesvirus protease dimer interface is capable of adopting alternative conformations, as the varicellar-zoster virus protease (which is a member of the herpesvirus family) shows an even larger reorganization 7 .…”

Section: Conformational Differencesmentioning

confidence: 91%

See 1 more Smart Citation

Conserved mode of peptidomimetic inhibition and substrate recognition of human cytomegalovirus protease

Tong

Qian

Massariol

et al. 1998

Nat Struct Mol Biol

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Human cytomegalovirus (HCMV) protease belongs to a new class of serine proteases, with a unique polypeptide backbone fold. The crystal structure of the protease in complex with a peptidomimetic inhibitor (based on the natural substrates and covering the P4 to P1' positions) has been determined at 2.7 A resolution. The inhibitor is bound in an extended conformation, forming an anti-parallel beta-sheet with the protease. The P3 and P1 side chains are less accessible to solvent, whereas the P4 and P2 side chains are more exposed. The inhibitor binding mode shows significant similarity to those observed for peptidomimetic inhibitors or substrates of other classes of serine proteases (chymotrypsin and subtilisin). HCMV protease therefore represents example of convergent evolution. In addition, large conformational differences relative to the structure of the free enzyme are observed, which may be important for inhibitor binding.

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Section: Conformational Differencesmentioning

confidence: 91%

“…There are two dimers of the protease in the asymmetric unit. This unit cell is related to that of the free enzyme reported by us earlier 3,11 .…”

Section: Methodsmentioning

confidence: 96%

Conserved mode of peptidomimetic inhibition and substrate recognition of human cytomegalovirus protease

Tong

Qian

Massariol

et al. 1998

Nat Struct Mol Biol

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“…2; Heras et al, 2003). Crystals of DsbG dehydrated in this way exhibited a dramatic improvement in diffraction quality, with the pattern improving from 10 Å to beyond 2 Å resolution (Table 2) Combining dehydration with other post-crystallization treatments such as annealing, soaking, cryocooling or rehydration has also resulted in spectacular improvements in the diffraction quality and resolution of protein crystals (Table 2) (Izard et al, 1997;Tong et al, 1997;Pang et al, 2002;Abergel, 2004). For example, a recent publication reported the dramatic improvement in diffraction resolution of three protein crystals upon annealing and dehydration [Escherichia coli YbgL from 12 to 2.6 Å , E. coli YggV (HAM1) from 12 to 2.6 Å and Candida albicans 3-dehydroquinate dehydratase from no diffraction to 3 Å ].…”

Section: Crystal Dehydrationmentioning

confidence: 99%

Post-crystallization treatments for improving diffraction quality of protein crystals

Heras

Martin

2005

Acta Crystallogr D Biol Cryst

198

183

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X-ray crystallography is the most powerful method for determining the three-dimensional structure of biological macromolecules. One of the major obstacles in the process is the production of high-quality crystals for structure determination. All too often, crystals are produced that are of poor quality and are unsuitable for diffraction studies. This review provides a compilation of post-crystallization methods that can convert poorly diffracting crystals into data-quality crystals. Protocols for annealing, dehydration, soaking and cross-linking are outlined and examples of some spectacular changes in crystal quality are provided. The protocols are easily incorporated into the structure-determination pipeline and a practical guide is provided that shows how and when to use the different post-crystallization treatments for improving crystal quality.

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“…Good results have been also obtained when protein crystals are mounted in a specific and adjustable stream of humidified gas, where it is possible to control the relative humidity [26,43–48,86–88]. Finally, crystal dehydration can also be performed by transferring the crystals into a dehydrating solution, which is the original mother liquor with a higher concentration of precipitant [24,27,50–70] or with a different dehydrating agent [49,71–85]. …”

Section: Resultsmentioning

confidence: 99%

Increasing the X-ray Diffraction Power of Protein Crystals by Dehydration: The Case of Bovine Serum Albumin and a Survey of Literature Data

Krauss

Sica

Mattia

et al. 2012

IJMS

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Serum albumin is one of the most widely studied proteins. It is the most abundant protein in plasma with a typical concentration of 5 g/100 mL and the principal transporter of fatty acids in plasma. While the crystal structures of human serum albumin (HSA) free and in complex with fatty acids, hemin, and local anesthetics have been characterized, no crystallographic models are available on bovine serum albumin (BSA), presumably because of the poor diffraction power of existing hexagonal BSA crystals. Here, the crystallization and diffraction data of a new BSA crystal form, obtained by the hanging drop method using MPEG 5K as precipitating agent, are presented. The crystals belong to space group C2, with unit-cell parameters a = 216.45 Å, b = 44.72 Å, c = 140.18 Å, β = 114.5°. Dehydration was found to increase the diffraction limit of BSA crystals from ~8 Å to 3.2 Å, probably by improving the packing of protein molecules in the crystal lattice. These results, together with a survey of more than 60 successful cases of protein crystal dehydration, confirm that it can be a useful procedure to be used in initial screening as a method of improving the diffraction limits of existing crystals.

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Experiences from the Structure Determination of Human Cytomegalovirus Protease

Cited by 8 publications

References 16 publications

Conserved mode of peptidomimetic inhibition and substrate recognition of human cytomegalovirus protease

Conserved mode of peptidomimetic inhibition and substrate recognition of human cytomegalovirus protease

Post-crystallization treatments for improving diffraction quality of protein crystals

Increasing the X-ray Diffraction Power of Protein Crystals by Dehydration: The Case of Bovine Serum Albumin and a Survey of Literature Data

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