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绵羊精子鞭毛中cAMP依赖性蛋白激酶的催化亚基具有独特的氨基末端序列。

The catalytic subunit of the cAMP-dependent protein kinase of ovine sperm flagella has a unique amino-terminal sequence.

作者信息

San Agustin J T, Leszyk J D, Nuwaysir L M, Witman G B

机构信息

Department of Cell Biology, University of Massachusetts Medical Center, Worcester Foundation Campus, Shrewsbury, Massachusetts 01545, USA.

出版信息

J Biol Chem. 1998 Sep 18;273(38):24874-83. doi: 10.1074/jbc.273.38.24874.

Abstract

The basis for the unusual properties of the catalytic subunit (C) of ram sperm cAMP-dependent protein kinase was investigated. Ram sperm C was purified and found by mass spectrometry (MS) to be approximately 890 Da smaller than Calpha, the predominant somatic isoform. Partial internal amino acid sequence from ram sperm C was an exact match to that of bovine Calpha, but differed from the predicted sequences for the Cbeta and Cgamma isoforms. MS analysis of 2-nitro-5-thiocyanatobenzoic acid fragments showed that the mass difference originated in the amino-terminal region. A unique blocked amino-terminal fragment was isolated from sperm C and sequenced by a combination of tandem mass spectrometry and Edman degradation of a subfragment. The results revealed that the amino-terminal myristate and the first 14 amino acids of Calpha are replaced by an amino-terminal acetate and six different amino acids in sperm C. The predicted mass difference due to these changes is 899 Da. The region of homology between sperm C and Calpha begins at the exon 1/exon 2 boundary in Calpha, suggesting that sperm C results from use of an alternate exon 1 in the Calpha gene. The different amino terminus of sperm C may be related to a unique requirement for localization of the "free" C subunit within the sperm flagellum.

摘要

对公羊精子环磷酸腺苷依赖性蛋白激酶催化亚基(C)异常特性的基础进行了研究。纯化了公羊精子C,通过质谱(MS)发现其比主要的体细胞亚型αC约小890 Da。公羊精子C的部分内部氨基酸序列与牛αC的序列完全匹配,但与预测的βC和γC亚型序列不同。对2-硝基-5-硫氰酸苯甲酸片段的MS分析表明,质量差异源于氨基末端区域。从精子C中分离出一个独特的封闭氨基末端片段,并通过串联质谱和亚片段的埃德曼降解相结合的方法进行测序。结果显示,精子C中氨基末端的肉豆蔻酸和αC的前14个氨基酸被氨基末端的乙酸盐和六个不同的氨基酸所取代。由于这些变化导致的预测质量差异为899 Da。精子C与αC之间的同源区域始于αC中的外显子1/外显子2边界,这表明精子C是由于在αC基因中使用了替代的外显子1而产生的。精子C不同的氨基末端可能与“游离”C亚基在精子鞭毛内定位的独特要求有关。

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