Multistep Denaturation of<i>Borrelia burgdorferi</i>OspA, a Protein Containing a Single-Layer β-Sheet

Koide, Shohei; Bu, Zimei; Risal, Dipesh; Pham, Thúy-Nga; Nakagawa, Tomoko; Tamura, A.; Engelman, Donald M.

doi:10.1021/bi982443+

Cited by 37 publications

(33 citation statements)

References 50 publications

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“…In greater detail, SEED decomposition of (i-iii) T4 phage lysozyme, α-lactalbumin, and OspA is consistent with the experimentally determined boundaries of intermediate structures (31)(32)(33)(34). (iv) β-Lactamase was found to unfold into two equilibrium intermediates with a concurrent decrease in the helical CD signal of each (35), consistent with SEED decomposition into a threedomain protein with two small partially helical domains.…”

Section: Qualifying Ratiosupporting

confidence: 75%

A thermodynamic definition of protein domains

Porter

Rose

2012

Proc. Natl. Acad. Sci. U.S.A.

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Protein domains are conspicuous structural units in globular proteins, and their identification has been a topic of intense biochemical interest dating back to the earliest crystal structures. Numerous disparate domain identification algorithms have been proposed, all involving some combination of visual intuition and/or structurebased decomposition. Instead, we present a rigorous, thermodynamically-based approach that redefines domains as cooperative chain segments. In greater detail, most small proteins fold with high cooperativity, meaning that the equilibrium population is dominated by completely folded and completely unfolded molecules, with a negligible subpopulation of partially folded intermediates. Here, we redefine structural domains in thermodynamic terms as cooperative folding units, based on m-values, which measure the cooperativity of a protein or its substructures. In our analysis, a domain is equated to a contiguous segment of the folded protein whose mvalue is largely unaffected when that segment is excised from its parent structure. Defined in this way, a domain is a self-contained cooperative unit; i.e., its cooperativity depends primarily upon intrasegment interactions, not intersegment interactions. Implementing this concept computationally, the domains in a large representative set of proteins were identified; all exhibit consistency with experimental findings. Specifically, our domain divisions correspond to the experimentally determined equilibrium folding intermediates in a set of nine proteins. The approach was also proofed against a representative set of 71 additional proteins, again with confirmatory results. Our reframed interpretation of a protein domain transforms an indeterminate structural phenomenon into a quantifiable molecular property grounded in solution thermodynamics.protein folding | protein structure | protein architecture | protein parsing D omains are visually arresting protein substructures with an influential history in protein biochemistry (1). These familiar, self-contained structural units were first noticed in some of the earliest solved protein structures (2, 3) and soon came to be recognized as common features of protein architecture (4).Dissecting proteins into their constituent domains provides a simple, intuitive approach to classifying protein structure, a molecular application of the time-honored principle of "carving nature at its joints" (5). Many structure-based computer algorithms have been devised to parse the ever-increasing number of solved proteins into discrete units; a highly abbreviated sample includes (6-13). Today, CATH (14) and SCOP (15) are the two most widely used domain classifications. Both are based on computational algorithms but rely ultimately on the human eye as the final arbiter of domain boundaries.However, seeing can be deceiving. The dependence on visual intuition introduces an unavoidable element of ambiguity into procedures for domain recognition. The most enduring domain definition, "potentially independent, stable folding uni...

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Section: Qualifying Ratiosupporting

confidence: 75%

A thermodynamic definition of protein domains

Porter

Rose

2012

Proc. Natl. Acad. Sci. U.S.A.

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“…A 66-residue, amino-terminally cystine-linked coiled coil derived from the leucine zipper region of the protein GCN4 was synthesized and purified by analogy to Choma et al (19). Staphylococcal nuclease (Snase), ␣ subunit of tryptophan synthase (␣-TS), and outer surface protein A (OspA) were gifts of D. Shortle (The Johns Hopkins University, Baltimore), O. Bilsel (University of Massachusetts Medical School, Worcester), C. R. Matthews (University of Massachusetts Medical School), and S. Koide (University of Chicago, Chicago) (6,20). Ubiquitin was expressed from the wild-type human expression vector pRSUB (Entrez gi576323), which was mutated (F45W), expressed, and purified as described in ref.…”

Section: Methodsmentioning

confidence: 99%

Random-coil behavior and the dimensions of chemically unfolded proteins

Kohn

Millett

Jacob

et al. 2004

Proc. Natl. Acad. Sci. U.S.A.

660

758

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Spectroscopic studies have identified a number of proteins that appear to retain significant residual structure under even strongly denaturing conditions. Intrinsic viscosity, hydrodynamic radii, and small-angle x-ray scattering studies, in contrast, indicate that the dimensions of most chemically denatured proteins scale with polypeptide length by means of the power-law relationship expected for random-coil behavior. Here we further explore this discrepancy by expanding the length range of characterized denatured-state radii of gyration (RG) and by reexamining proteins that reportedly do not fit the expected dimensional scaling. We find that only 2 of 28 crosslink-free, prosthetic-group-free, chemically denatured polypeptides deviate significantly from a power-law relationship with polymer length. The RG of the remaining 26 polypeptides, which range from 16 to 549 residues, are well fitted (r2 = 0.988) by a power-law relationship with a best-fit exponent, 0.598 ± 0.028, coinciding closely with the 0.588 predicted for an excluded volume random coil. Therefore, it appears that the mean dimensions of the large majority of chemically denatured proteins are effectively indistinguishable from the mean dimensions of a random-coil ensemble

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“…The determined R g is within the range observed for other proteins of similar length. For example, the ␣-subunit tryptophan synthase is 268 residues long and has an R g of 19.1 Å, whereas OspA has an R g of 25.0 Å and is 257 residues long (44,45). A homodimer of E4-ORF3 contains 272 amino acid residues, including the unstructured residues in the His 6 tag.…”

Section: His 6 -Tev-tagged E4-orf3 Protein Is Functional In Vivo and mentioning

confidence: 99%

Biophysical and Functional Analyses Suggest That Adenovirus E4-ORF3 Protein Requires Higher-order Multimerization to Function against Promyelocytic Leukemia Protein Nuclear Bodies

Patsalo

Yondola

Luan

et al. 2012

Journal of Biological Chemistry

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Background:The adenovirus E4-ORF3 protein disrupts PML nuclear bodies to inhibit antiviral activity. Results: The WT E4-ORF3 protein forms higher-order multimers, whereas a nonfunctional mutant forms a dimer. Conclusion: E4-ORF3 protein multimerization likely is required for the activity of this protein.Significance: These results provide new insight into the properties of the adenovirus E4-ORF3 protein and suggest that higher-order protein multimerization is essential for activity.

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Multistep Denaturation ofBorrelia burgdorferiOspA, a Protein Containing a Single-Layer β-Sheet

Cited by 37 publications

References 50 publications

A thermodynamic definition of protein domains

A thermodynamic definition of protein domains

Random-coil behavior and the dimensions of chemically unfolded proteins

Biophysical and Functional Analyses Suggest That Adenovirus E4-ORF3 Protein Requires Higher-order Multimerization to Function against Promyelocytic Leukemia Protein Nuclear Bodies

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