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拟南芥液泡ATP酶“57 kDa”核苷酸结合亚基的cDNA序列及同源性

cDNA sequence and homologies of the "57-kDa" nucleotide-binding subunit of the vacuolar ATPase from Arabidopsis.

作者信息

Manolson M F, Ouellette B F, Filion M, Poole R J

机构信息

Department of Biology, McGill University, Montreal, Quebec, Canada.

出版信息

J Biol Chem. 1988 Dec 5;263(34):17987-94.

PMID:2903860
Abstract

Functional and structural similarities among a wide variety of endomembrane H+-ATPases suggest that they form a distinct class with a common origin. Immunological studies (Manolson, M. F., Percy, J. M., Apps, D. K., Xie, X. S., Stone, D. K., and Poole, R. J. (1987) in Proceedings of the Membrane Protein Symposium (Goheen, S. C., ed) pp. 427-434, Bio-Rad, Richmond, CA, and M. F. Manolson, J. M. Percy, D. K. Apps, X. S. Xie, D. K. Stone, M. Harrison, D. J. Clarke, R. J. Poole, unpublished data) support this idea and suggest an evolutionary relationship between the endomembrane and F0F1 ATPases. Further examination of relationships necessitates comparison of protein/nucleic acid sequence data. To this end, we have cloned and sequenced the cDNA encoding the 57-kDa polypeptide of the Arabidopsis vacuolar membrane H+-ATPase. To our knowledge, this is the first report of the sequence of a "57-kDa" subunit for plant or animal endomembrane H+-ATPase. This cDNA encodes a hydrophilic polypeptide containing a putative ATP binding site. Lack of a secretion signal sequence suggests it is not processed through the endoplasmic reticulum but translated on cytosolic ribosomes. Comparison of protein sequences shows the 57-kDa subunit from Arabidopsis to be nearly identical with the corresponding subunit in Neurospora vacuolar membrane H+-ATPase, very similar to the beta subunit of the archaebacterium Sulfolobus, and slightly, but nevertheless significantly, homologous to the alpha and beta subunits of the F0F1-ATPases. These results suggest that these different classes of ATPases have evolved from a common ancestor.

摘要

多种内膜H⁺ -ATP酶之间的功能和结构相似性表明,它们形成了一个具有共同起源的独特类别。免疫学研究(Manolson, M. F., Percy, J. M., Apps, D. K., Xie, X. S., Stone, D. K., and Poole, R. J. (1987) 发表于《膜蛋白研讨会论文集》(Goheen, S. C. 主编)第427 - 434页,Bio - Rad,加利福尼亚州里士满,以及M. F. Manolson, J. M. Percy, D. K. Apps, X. S. Xie, D. K. Stone, M. Harrison, D. J. Clarke, R. J. Poole,未发表数据)支持了这一观点,并表明内膜和F₀F₁ -ATP酶之间存在进化关系。对这种关系的进一步研究需要比较蛋白质/核酸序列数据。为此,我们克隆并测序了编码拟南芥液泡膜H⁺ -ATP酶57 kDa多肽的cDNA。据我们所知,这是关于植物或动物内膜H⁺ -ATP酶“57 kDa”亚基序列的首次报道。该cDNA编码一种含有假定ATP结合位点的亲水性多肽。缺乏分泌信号序列表明它不是通过内质网加工的,而是在胞质核糖体上翻译的。蛋白质序列比较显示,拟南芥的57 kDa亚基与粗糙脉孢菌液泡膜H⁺ -ATP酶中的相应亚基几乎相同,与嗜热栖热菌的β亚基非常相似,并且与F₀F₁ -ATP酶的α和β亚基有轻微但显著的同源性。这些结果表明,这些不同类别的ATP酶是从一个共同祖先进化而来的。

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