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平滑肌肌球蛋白轻链磷酸酶小非催化亚基的同工型。

Isoforms of the small non-catalytic subunit of smooth muscle myosin light chain phosphatase.

作者信息

Mabuchi K, Gong B J, Langsetmo K, Ito M, Nakano T, Tao T

机构信息

Muscle Research Group, Boston Biomedical Research Institute, 20 Staniford Street, Boston, MA 02114, USA.

出版信息

Biochim Biophys Acta. 1999 Oct 12;1434(2):296-303. doi: 10.1016/s0167-4838(99)00182-x.

Abstract

Chicken gizzard smooth muscle myosin light chain phosphatase is composed of a approximately 37 kDa catalytic subunit, a approximately 110 kDa myosin binding or targeting subunit and a approximately 20 kDa subunit (MPs) whose function is as yet undefined. It was reported previously that a cloned chicken gizzard MPs cDNA encodes a protein of 186 amino acids (aa) [Y.H. Chen, M.X. Chen, D.R. Alessi, D.G. Gampbell, C. Shanahan, P. Cohen, P.T.W. Cohen, FEBS Lett. 356 (1994) 51-55]. More recently, we obtained by PCR amplification another MPs cDNA that encodes a protein of only 161 aa [Y. Zhang, K. Mabuchi, T. Tao, Biochim. Biophys. Acta 1343 (1997) 51-58]. In this work we obtained cDNAs corresponding to both sequences using a different set of PCR primers, indicating that the two sequences correspond to isoforms that most likely arose from alternative splicing of the same gene. Using two polyclonal antibodies, one raised against the recombinant 161 aa isoform of chicken gizzard MPs and the other against a C-terminal polypeptide that is present only in the 186 aa isoform, we found that while the 161 aa isoform is the predominant one in chicken gizzard, in chicken aorta it is the 186 aa one; in chicken stomach both isoforms are present, and in mammalian tissues such as ferret and rat only the 186 aa isoform is detected. Furthermore, we purified the MPs associated with the chicken gizzard myosin light chain phosphatase holoenzyme and determined its molecular weight, amino acid composition and six residues of its C-terminal sequence. The results from these analyses showed conclusively that the predominant isoform in chicken gizzard is the 161 aa one.

摘要

鸡胗平滑肌肌球蛋白轻链磷酸酶由一个约37 kDa的催化亚基、一个约110 kDa的肌球蛋白结合或靶向亚基以及一个功能尚未明确的约20 kDa亚基(MPs)组成。先前有报道称,克隆的鸡胗MPs cDNA编码一种含186个氨基酸(aa)的蛋白质[Y.H. Chen,M.X. Chen,D.R. Alessi,D.G. Gampbell,C. Shanahan,P. Cohen,P.T.W. Cohen,FEBS Lett. 356 (1994) 51 - 55]。最近,我们通过PCR扩增获得了另一个MPs cDNA,它编码一种仅含161个aa的蛋白质[Y. Zhang,K. Mabuchi,T. Tao,Biochim. Biophys. Acta 1343 (1997) 51 - 58]。在这项工作中,我们使用不同的一组PCR引物获得了与这两个序列对应的cDNA,表明这两个序列对应于最有可能由同一基因的可变剪接产生的同工型。使用两种多克隆抗体,一种针对鸡胗MPs的重组161 aa同工型制备,另一种针对仅存在于186 aa同工型中的C末端多肽制备,我们发现虽然161 aa同工型是鸡胗中的主要同工型,但在鸡主动脉中是186 aa同工型;在鸡胃中两种同工型都存在,而在雪貂和大鼠等哺乳动物组织中仅检测到186 aa同工型。此外,我们纯化了与鸡胗肌球蛋白轻链磷酸酶全酶相关的MPs,并测定了其分子量、氨基酸组成及其C末端序列的六个残基。这些分析结果确凿地表明,鸡胗中的主要同工型是161 aa的那种。

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