Aram M. Nersissian
University of California, Los Angeles
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Featured researches published by Aram M. Nersissian.
Journal of Biological Chemistry | 2000
Joy J. Goto; Haining Zhu; Raylene J. Sanchez; Aram M. Nersissian; Edith Butler Gralla; Joan Selverstone Valentine; Diane E. Cabelli
The presence of the copper ion at the active site of human wild type copper-zinc superoxide dismutase (CuZnSOD) is essential to its ability to catalyze the disproportionation of superoxide into dioxygen and hydrogen peroxide. Wild type CuZnSOD and several of the mutants associated with familial amyotrophic lateral sclerosis (FALS) (Ala4 → Val, Gly93 → Ala, and Leu38 → Val) were expressed inSaccharomyces cerevisiae. Purified metal-free (apoproteins) and various remetallated derivatives were analyzed by metal titrations monitored by UV-visible spectroscopy, histidine modification studies using diethylpyrocarbonate, and enzymatic activity measurements using pulse radiolysis. From these studies it was concluded that the FALS mutant CuZnSOD apoproteins, in direct contrast to the human wild type apoprotein, have lost their ability to partition and bind copper and zinc ions in their proper locations in vitro. Similar studies of the wild type and FALS mutant CuZnSOD holoenzymes in the “as isolated” metallation state showed abnormally low copper-to-zinc ratios, although all of the copper acquired was located at the native copper binding sites. Thus, the copper ions are properly directed to their native binding sites in vivo, presumably as a result of the action of the yeast copper chaperone Lys7p (yeast CCS). The loss of metal ion binding specificity of FALS mutant CuZnSODsin vitro may be related to their role in ALS.
Journal of Biological Chemistry | 2008
Bryan F. Shaw; Herman Lelie; Armando Durazo; Aram M. Nersissian; Guillan Xu; Pik K. Chan; Edith Butler Gralla; Ashutosh Tiwari; Lawrence J. Hayward; David R. Borchelt; Joan Selverstone Valentine; Julian P. Whitelegge
Determining the composition of aggregated superoxide dismutase 1 (SOD1) species associated with amyotrophic lateral sclerosis (ALS), especially with respect to co-aggregated proteins and post-translational modifications, could identify cellular or biochemical factors involved in the formation of these aggregates and explain their apparent neurotoxicity. The results of mass spectrometric and shotgun-proteomic analyses of SOD1-containing aggregates isolated from spinal cords of symptomatic transgenic ALS mice using two different isolation strategies are presented, including 1) resistance to detergent extraction and 2) size exclusion-coupled anti-SOD1 immunoaffinity chromatography. Forty-eight spinal cords from three different ALS-SOD1 mutant mice were analyzed, namely G93A, G37R, and the unnatural double mutant H46R/H48Q. The analysis consistently revealed that the most abundant proteins recovered from aggregate species were full-length unmodified SOD1 polypeptides. Although aggregates from some spinal cord samples contained trace levels of highly abundant proteins, such as vimentin and neurofilament-3, no proteins were consistently found to co-purify with mutant SOD1 in stoichiometric quantities. The results demonstrate that the principal protein in the high molecular mass aggregates whose appearance correlates with symptoms of the disease is the unmodified, full-length SOD1 polypeptide.
Journal of Biological Chemistry | 2006
Bryan F. Shaw; Armando Durazo; Aram M. Nersissian; Julian P. Whitelegge; Kym F. Faull; Joan Selverstone Valentine
Hydrogen exchange monitored by mass spectrometry has been used to study the structural behavior of the pathogenic A4V variant of superoxide dismutase 1 (SOD1) in the metal-free (apo) form. Mass spectrometric data revealed that in the disulfide-intact (S-S) form, the A4V variant is destabilized at residues 50-53, in the disulfide subloop of the dimer interface, but many other regions of the A4V protein exhibited hydrogen exchange properties identical to that of the wild type protein. Additionally, mass spectrometry revealed that A4V apoSOD1S-S undergoes slow localized unfolding in a large segment of the β-barrel that included β3, β4, and loops II and III. In the disulfide-reduced form, A4V apoSOD1 exchanged like a “random coil” polypeptide at 20 °C and began to populate folded states at 4 °C. These local and global unfolding events could facilitate intermolecular protein-protein interactions that cause the aggregation or neurotoxicity of A4V SOD1.
Journal of Biological Inorganic Chemistry | 2000
T. J. Lyons; Aram M. Nersissian; H. Huang; H. Yeom; C. R. Nishida; Janet A. Graden; Edith Butler Gralla; Joan Selverstone Valentine
Abstract We have investigated factors that influence the properties of the zinc binding site in yeast copper-zinc superoxide dismutase (CuZnSOD). The properties of yeast CuZnSOD are essentially invariant from pH 5 to pH 9. However, below this pH range there is a change in the nature of the zinc binding site which can be interpreted as either (1) a change in metal binding affinity from strong to weak, (2) the expulsion of the metal bound at this site, or (3) a transition from a normal distorted tetrahedral ligand orientation to a more symmetric arrangement of ligands. This change is strongly reminiscent of a similar pH-induced transition seen for the bovine protein and, based on the data presented herein, is proposed to be a property that is conserved among CuZnSODs. The transition demonstrated for the yeast protein is not only sensitive to the pH of the buffering solution but also to the occupancy and redox status of the adjacent copper binding site. Furthermore, we have investigated the effect of single site mutations on the pH- and redox-sensitivity of Co2+ binding at the zinc site. Each of the mutants H46R, H48Q, H63A, H63E, H80C, G85R, and D83H is capable of binding Co2+ to a zinc site with a distorted tetrahedral geometry similar to that of wild-type. However, they do so only if Cu+ is bound at the copper site or if the pH in raised to near physiological levels, indicating that the change at the zinc binding site seen in the wild-type is conserved in the mutants, albeit with an altered pKa. The mutants H71C and D83A did not bind Co2+ in a wild-type-like fashion under any of the conditions tested. This study reveals that the zinc binding site is exquisitely sensitive to changes in the protein environment. Since three of the mutant yeast proteins investigated here contain mutations analogous to those that cause ALS (amyotrophic lateral sclerosis) in humans, this finding implicates improper metal binding as a mechanism by which CuZnSOD mutants exert their toxic gain of function.
Advances in Protein Chemistry | 2002
Aram M. Nersissian; Eric Shipp
Publisher Summary This chapter introduces the blue copper-binding (BCB) domain-containing proteins based on the analysis of the genomic and expressed sequence tag (EST) sequence data, and presents the classification system. This classification is based on their ability to bind copper and the specific features of their domain organization. Members of the first three classes harbor single or multiple type 1, blue copper-binding sites, while members of the fourth class do not appear to bind copper. Some analysis of codon usage for conserved amino acids involved in copper binding will be used to trace the evolutionary history of the blue copper-binding (BCB) domains within a single genorne. The chapter also discusses the structural and physical characteristics of each kind of blue copper-binding (BCB) domain protein. The large number of blue copper-binding (BCB) domain proteins in plants may be explained by the phenomenon of genome duplication, believed to occur widely in the plant kingdom, as well as by different lateral gene transfers The blue copper-binding (BCB) domain-containing proteins evolved by gene duplication and fusion with other structural modules, resulting in diverse subcellular localization and the ability to carry out complex reactions that often differ from that of the ancestral protein. They are also modified by extensive amino acid substitutions and insertions.
Journal of Biological Chemistry | 2009
Armando Durazo; Bryan F. Shaw; Madhuri Chattopadhyay; Kym F. Faull; Aram M. Nersissian; Joan Selverstone Valentine; Julian P. Whitelegge
The structure and unfolding of metal-free (apo) human wild-type SOD1 and three pathogenic variants of SOD1 (A4V, G93R, and H48Q) that cause familial amyotrophic lateral sclerosis have been studied with amide hydrogen/deuterium exchange and mass spectrometry. The results indicate that a significant proportion of each of these proteins exists in solution in a conformation in which some strands of the β-barrel (i.e. β2) are well protected from exchange at physiological temperature (37 °C), whereas other strands (i.e. β3 and β4) appear to be unprotected from hydrogen/deuterium exchange. Moreover, the thermal unfolding of these proteins does not result in the uniform incorporation of deuterium throughout the polypeptide but involves the local unfolding of different residues at different temperatures. Some regions of the proteins (i.e. the “Greek key” loop, residues 104–116) unfold at a significantly higher temperature than other regions (i.e. β3 and β4, residues 21–53). Together, these results show that human wild-type apo-SOD1 and variants have a partially unfolded β-barrel at physiological temperature and unfold non-cooperatively.
Biochemistry | 1999
P. John Hart; Melinda Balbirnie; Nancy L. Ogihara; Aram M. Nersissian; Manfred S. Weiss; Joan Selverstone Valentine; David Eisenberg
Proceedings of the National Academy of Sciences of the United States of America | 1996
Thomas J. Lyons; Hongbin Liu; Joy J. Goto; Aram M. Nersissian; James A. Roe; Janet A. Graden; Carla Cafe; Dale E. Bredesen; Edith Butler Gralla; Joan Selverstone Valentine
Proceedings of the National Academy of Sciences of the United States of America | 2005
Jorge A. Rodriguez; Bryan F. Shaw; Armando Durazo; Se Hui Sohn; Peter A. Doucette; Aram M. Nersissian; Kym F. Faull; Daryl K. Eggers; Ashutosh Tiwari; Lawrence J. Hayward; Joan Selverstone Valentine
Protein Science | 1998
Aram M. Nersissian; C. Immoos; Michael G. Hill; P. J. Hart; G. Williams; R. G. Herrmann; Joan Selverstone Valentine