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肌球蛋白亚片段1中配体诱导的构象扰动研究。使用光探针检测SH2和SH1巯基周围的环境。

Studies of ligand-induced conformational perturbations in myosin subfragment 1. An examination of the environment about the SH2 and SH1 thiols using a photoprobe.

作者信息

Rajasekharan K N, Mayadevi M, Burke M

机构信息

Department of Biology, Case Institute of Technology, Case Western Reserve University, Cleveland, Ohio 44106.

出版信息

J Biol Chem. 1989 Jun 25;264(18):10810-9.

PMID:2732248
Abstract

The effect of ligand binding on the environment near the SH2 and SH1 thiols in myosin subfragment 1 has been investigated by photocross-linking after specific labeling of these thiols individually with 4-(N-maleimido)benzophenone (MBP). On photolysis, cross-linking occurred from SH2-MBP to the middle 50-kDa segment, and subsequent immunopeptide mapping revealed that the cross-link was made to a peptide stretch 31-32 kDa from the N terminus in the absence of MgADP, whereas in its presence the cross-link occurred at about 60-61 kDa from the N terminus. Photolysis of SH1-MBP in the absence of MgADP resulted in a major cross-link to the 27-kDa N-terminal segment and minor cross-links to the 50-kDa middle segment. In the presence of MgADP, no new cross-link occurred but the amount of cross-linking to the 50-kDa segment increased at the expense of the other. Immunopeptide mapping indicated that the regions in the 27- and 50-kDa peptides that were cross-linked to SH1-MBP are at about 14-16 and 55-56 kDa from the N terminus respectively. These results indicate that when nucleotide binds to S1, SH2 is displaced relative to the 50-kDa segment, whereas the local environment around SH1 does not change significantly because photolysis in the presence of MgADP resulted in a change at the site of cross-linking for SH2-MBP but caused only a redistribution of the relative amounts of the cross-links formed from SH1-MBP.

摘要

通过用4-(N-马来酰亚胺)二苯甲酮(MBP)分别对肌球蛋白亚片段1中的SH2和SH1硫醇进行特异性标记后进行光交联,研究了配体结合对这些硫醇附近环境的影响。光解时,交联发生在SH2-MBP与中间50 kDa片段之间,随后的免疫肽图谱显示,在没有MgADP的情况下,交联发生在距N端31-32 kDa的肽段,而在其存在的情况下,交联发生在距N端约60-61 kDa处。在没有MgADP的情况下,SH1-MBP的光解导致与27 kDa N端片段的主要交联以及与50 kDa中间片段的次要交联。在MgADP存在的情况下,没有发生新的交联,但与50 kDa片段的交联量增加,而其他交联量减少。免疫肽图谱表明,与SH1-MBP交联的27 kDa和50 kDa肽段中的区域分别距N端约14-16 kDa和55-56 kDa。这些结果表明,当核苷酸与S1结合时,SH2相对于50 kDa片段发生位移,而SH1周围的局部环境没有明显变化,因为在MgADP存在下的光解导致SH2-MBP交联位点发生变化,但仅导致SH1-MBP形成的交联相对量的重新分布。

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