Marina Bukhtiyarova scite author profile

catalyst can operate in a stable way without the presence of carbon monoxide in the feed, which means that increased water contents in the product gas cannot destroy the catalyst's performance completely. The presence of benzene in the feed does not lead to a deactivation of the catalyst. With these findings methanol production starting from exhaust gases from steel mills seems to become an interesting alternative for sustainable methanol production.Abstract CO 2 hydrogenation as a route for the chemical energy storage over a commercial Cu/ZnO/Al 2 O 3 catalyst has been studied. To check the optimal conditions for an efficient methanol production the influence of temperature and space velocity on the catalytic performance has been demonstrated. Time-on-stream measurements in the absence and the presence of benzene in the gas feed mixture were performed to investigate the possibility to use alternative carbon sources, which contain traces of aromatics. The

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Complete nucleotide sequence of pSMB 74, a plasmid encoding the production of pediocin AcH in Pediococcus acidilactici

Motlagh

Bukhtiyarova

Ray

1994

Lett Appl Microbiol

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Several Pediococcus acidilactici strains produce a plasmid-encoded bacteriocin, pediocin AcH. Previous studies have shown that this plasmid, designated as pSMB 74, encodes genes associated with the production of prepediocin, its post-translation processing to pediocin AcH, transmembrane translocation of these molecules, and immunity of producer cells against pediocin AcH. We report here the complete nucleotide sequence of pSMB 74. The plasmid has a total of 8877 bp. Four genes have been located on pSMB 74. The genes are arranged in a gene cluster of 3500 bp and share a common promoter and rho-independent stem-loop terminator. The four genes, each with independent ribosome binding sites (rbs), initiation and termination codons and spacer sequences in between, were designated as pap A, pap B, pap C and pap D and encode respectively for proteins of 62, 112, 174 and 724 amino acids. The results of this study can be useful either to introduce a suitable marker at a unique restriction site in pSMB 74 and use it as a vector or to clone the pap gene cluster in a suitable plasmid and transform desirable strains for pediocin AcH production. The gene sequence has been submitted to Gene Bank (Acc. No. U02482).

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A Continuous Fluorescence-Based Assay of Human Cytomegalovirus Protease Using a Peptide Substrate

Holskin

Bukhtiyarova

Dunn

et al. 1995

Analytical Biochemistry

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Analysis of Imatinib and Sorafenib Binding to p38α Compared with c-Abl and b-Raf Provides Structural Insights for Understanding the Selectivity of Inhibitors Targeting the DFG-Out Form of Protein Kinases

Namboodiri¹,

Bukhtiyarova²,

Ramcharan³

et al. 2010

Biochemistry

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Protein kinases c-Abl, b-Raf, and p38alpha are recognized as important targets for therapeutic intervention. c-Abl and b-Raf are major targets of marketed oncology drugs Imatinib (Gleevec) and Sorafenib (Nexavar), respectively, and BIRB-796 is a p38alpha inhibitor that reached Phase II clinical trials. A shared feature of these drugs is the fact that they bind to the DFG-out forms of their kinase targets. Although the discovery of this class of kinase inhibitors has increased the level of emphasis on the design of DFG-out inhibitors, the structural determinants for their binding and stabilization of the DFG-out conformation remain unclear. To improve our understanding of these determinants, we determined cocrystal structures of Imatinib and Sorafenib with p38alpha. We also conducted a detailed analysis of Imatinib and Sorafenib binding to p38alpha in comparison with BIRB-796, including binding kinetics, binding interactions, the solvent accessible surface area (SASA) of the ligands, and stabilization of key structural elements of the protein upon ligand binding. Our results yield an improved understanding of the structural requirements for stabilizing the DFG-out form and a rationale for understanding the genesis of ligand selectivity among DFG-out inhibitors of protein kinases.

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