Metal-binding properties of human centrin-2 determined by micro-electrospray ionization mass spectrometry and UV spectroscopy

Craig, Theodore A.; Benson, Linda M.; Bergen, H. Robert; Venyaminov, Sergei Yu.; Salisbury, Jeffrey L.; Ryan, Zachary C.; Thompson, James R.; Sperry, Justin B.; Gross, Michael L.; Kumar, Rajiv

doi:10.1016/j.jasms.2006.04.029

Cited by 18 publications

(16 citation statements)

References 84 publications

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“…Protein concentration was determined conventionally by absorbance at 277 nm using an E m M ϭ 1.46 mM Ϫ1 cm Ϫ1 and after purification by the Bio-Rad (Bradford) method (28). Native HsCen-2-HsCen-2 was expressed and purified as described earlier (29). Crystallization trials were conducted using hanging drop vapor diffusion methods with over 3000 crystallization solutions, which were then optimized for the production of large single crystals.…”

Section: Methodsmentioning

confidence: 99%

“…Titrating HsCen-2 (26,43) and other centrins (44) to Ca 2ϩ saturation is complicated by aggregation of high order oligomers, an aggregation of reversible nature. Deletion of amino acids 1-24 has little effect on protein stability, global secondary structure, or metal binding (29) but does prevent aggregation; thus, these residues must be involved in the self-assembly (45). The formation of fibers consisting of centrin may be of physiological importance in the duplication and segregation of microtubule organizing centers (21).…”

Section: Disordered Hscen-2 N-terminalmentioning

confidence: 99%

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The Structure of the Human Centrin 2-Xeroderma Pigmentosum Group C Protein Complex

Thompson

Ryan

Salisbury

et al. 2006

Journal of Biological Chemistry

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117

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Human centrin-2 plays a key role in centrosome function and stimulates nucleotide excision repair by binding to the xeroderma pigmentosum group C protein. To determine the structure of human centrin-2 and to develop an understanding of molecular interactions between centrin and xeroderma pigmentosum group C protein, we characterized the crystal structure of calcium-loaded full-length centrin-2 complexed with a xeroderma pigmentosum group C peptide. Our structure shows that the carboxyl-terminal domain of centrin-2 binds this peptide and two calcium atoms, whereas the amino-terminal lobe is in a closed conformation positioned distantly by an ordered ␣-helical linker. A stretch of the amino-terminal domain unique to centrins appears disordered. Two xeroderma pigmentosum group C peptides both bound to centrin-2 also interact to form an ␣-helical coiled-coil. The interface between centrin-2 and each peptide is predominantly nonpolar, and key hydrophobic residues of XPC have been identified that lead us to propose a novel binding motif for centrin.Human centrin-2 (HsCen-2) 2 is a Ca 2ϩ -binding protein of the calmodulin-parvalbumin EF-hand superfamily (2, 3). HsCen-2 and two other human centrins (4) are best known for functions outside the nucleus. Centrins have essential roles in the duplication and segregation of microtubule organizing centers (5, 6). Much research has focused on these functions, because abnormal centrosome duplication may lead to chromosomal instability and then cancer, an idea supported by discovery of supernumerary abnormal centrosomes in different human tumor cells (7-10). In addition to its role in centrosome function, HsCen-2 is found as a stabilizing component of xeroderma pigmentosum complement protein C (XPC) and HRad23B complexes (11,12). The XPCcontaining heterotrimer is involved in recognition of DNA lesions and initiation of global genome nucleotide excision repair. Global genome nucleotide excision repair is an important DNA repair pathway for damage caused by UV radiation, carcinogens, and chemotherapeutic agents, and impairment of XPC function is associated with the genetic disorder xeroderma pigmentosum. HsCen-2 appears to promote DNA binding by XPC both in vivo and in vitro and increases the specificity of the heterotrimer for damaged DNA (12, 13). The mechanism by which HsCen-2 binds to XPC is not understood.Centrins are also involved in cilia function (14). Moreover, Ca 2ϩ -triggered assembly of HsCen-1 and transducin appears to regulate transducin translocation through the connecting cilium of vertebrate photoreceptors (15)(16)(17)(18). Whereas the first centrin, also known as caltractin (Cdc31p), was found in fibers linking the flagellar apparatus to the nuclei of Tetraselmis striata green alga (19), homologs have since been identified in many organisms, including fungi, plants, and higher eukaryotes. Functional similarities between centrins from various species seem likely. For example, Ca 2ϩ -induced contractions of a fiber formed by caltractin and Sfi1p are thought to play ...

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Section: Methodsmentioning

confidence: 99%

Section: Disordered Hscen-2 N-terminalmentioning

confidence: 99%

The Structure of the Human Centrin 2-Xeroderma Pigmentosum Group C Protein Complex

Thompson

Ryan

Salisbury

et al. 2006

Journal of Biological Chemistry

Self Cite

117

View full text Add to dashboard Cite

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“…Electrospray ionization mass spectrometry (ESI-MS) is a well established method for characterizing protein structural transition (Hooke et al 1995;Konermann 2004;Kaltashov and Eyles 2005;Craig et al 2006). The technique has also been applied in studying the amyloid fibrillation of amyloidogenic proteins, lysozyme in particular (Nettleton and Robinson, 2000;Caddy and Robinson 2006).…”

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confidence: 99%

The first step of hen egg white lysozyme fibrillation, irreversible partial unfolding, is a two‐state transition

Shashilov

Ermolenkov

et al. 2007

Protein Science

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Amyloid fibril depositions are associated with many neurodegenerative diseases as well as amyloidosis. The detailed molecular mechanism of fibrillation is still far from complete understanding. In our previous study of in vitro fibrillation of hen egg white lysozyme, an irreversible partially unfolded intermediate was characterized. A similarity of unfolding kinetics found for the secondary and tertiary structure of lysozyme using deep UV resonance Raman (DUVRR) and tryptophan fluorescence spectroscopy leads to a hypothesis that the unfolding might be a two-state transition. In this study, chemometric analysis, including abstract factor analysis (AFA), target factor analysis (TFA), evolving factor analysis (EFA), multivariate curve resolutionalternating least squares (ALS), and genetic algorithm, was employed to verify that only two principal components contribute to the DUVRR and fluorescence spectra of soluble fraction of lysozyme during the fibrillation process. However, a definite conclusion on the number of conformers cannot be made based solely on the above spectroscopic data although chemometric analysis suggested the existence of two principal components. Therefore, electrospray ionization mass spectrometry (ESI-MS) was also utilized to address the hypothesis. The protein ion charge state distribution (CSD) envelopes of the incubated lysozyme were well fitted with two principal components. Based on the above analysis, the partial unfolding of lysozyme during in vitro fibrillation was characterized quantitatively and proven to be a two-state transition. The combination of ESI-MS and Raman and fluorescence spectroscopies with advanced statistical analysis was demonstrated to be a powerful methodology for studying protein structural transformations.

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“…Structure prediction analysis (14), limited proteolysis (14), and NMR (37) identified several highly disordered regions: the N terminus (residues 1-154), the C terminus (residues 816-940), and a loop inserted into the TGD domain comprising residues 331-517. Finally, CETN2 may also contribute to this overall flexibility, because it can adopt different conformations depending on its metal-binding state (38); however, the resolution of the XPC-RAD23B subcomplex was not markedly improved, suggesting that this contribution to complex flexibility is minor, as would be expected for its relatively small mass contribution to the complex. The recently described requirement of RNA for the XPC complex to interact with its transcription partner SOX2 (25) invokes the idea of low-complexity domains or regions, perhaps interspersed throughout XPC, linking their inherent flexibility to a critical aspect of the XPC complex's function.…”

Section: Discussionmentioning

confidence: 99%

Architecture of the human XPC DNA repair and stem cell coactivator complex

Zhang

Grob

et al. 2015

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

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The Xeroderma pigmentosum complementation group C (XPC) complex is a versatile factor involved in both nucleotide excision repair and transcriptional coactivation as a critical component of the NANOG, OCT4, and SOX2 pluripotency gene regulatory network. Here we present the structure of the human holo-XPC complex determined by single-particle electron microscopy to reveal a flexible, ear-shaped structure that undergoes localized loss of order upon DNA binding. We also determined the structure of the complete yeast homolog Rad4 holo-complex to find a similar overall architecture to the human complex, consistent with their shared DNA repair functions. Localized differences between these structures reflect an intriguing phylogenetic divergence in transcriptional capabilities that we present here. Having positioned the constituent subunits by tagging and deletion, we propose a model of key interaction interfaces that reveals the structural basis for this difference in functional conservation. Together, our findings establish a framework for understanding the structure-function relationships of the XPC complex in the interplay between transcription and DNA repair.transcription | stem cells | DNA repair | structure | biochemistry

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Metal-binding properties of human centrin-2 determined by micro-electrospray ionization mass spectrometry and UV spectroscopy

Cited by 18 publications

References 84 publications

The Structure of the Human Centrin 2-Xeroderma Pigmentosum Group C Protein Complex

The Structure of the Human Centrin 2-Xeroderma Pigmentosum Group C Protein Complex

The first step of hen egg white lysozyme fibrillation, irreversible partial unfolding, is a two‐state transition

Architecture of the human XPC DNA repair and stem cell coactivator complex

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