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酵母中的分泌:前体蛋白与膜受体的结合以及ATP依赖性转运在体外是相继且可分离的事件。

Secretion in yeast: preprotein binding to a membrane receptor and ATP-dependent translocation are sequential and separable events in vitro.

作者信息

Sanz P, Meyer D I

机构信息

Department of Biological Chemistry, University of California, Los Angeles School of Medicine 90024.

出版信息

J Cell Biol. 1989 Jun;108(6):2101-6. doi: 10.1083/jcb.108.6.2101.

DOI:10.1083/jcb.108.6.2101
PMID:2544601
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2115617/
Abstract

We have used a cytosol-free assay in which efficient translocation and signal peptide cleavage is achieved when the affinity-purified precursor of OmpA (proOmpA) is diluted out of 8 M urea into a suspension of yeast rough microsomes. This aspect of protein targeting and transport occurs in two discernible steps: (a) in the absence of ATP and cytosolic factors, the precursor binds to the membranes but is not translocated; (b) addition of ATP results in the translocation of the bound precursor and its processing to the mature form. The binding to microsomes of radiolabeled proOmpA is saturable and inhibited by the addition of unlabeled proOmpA but not by mature OmpA or other proteins. The binding of radiolabeled prepro-alpha-factor is also effectively competed by other preproteins, but not by mature ones. Scatchard analysis showed the Kd of proOmpA to be 7.5 X 10(-9) M. Binding is most likely protein mediated as treatment of the microsomes with the protease papain was found to be inhibitory. These results represent the first functional characterization of secretory protein precursor binding to membranes. Alkylation of the microsomes with NEM, washing the membranes with urea or using membranes from the (translocation) mutant ptll at the nonpermissive temperature, did not affect binding, but did eliminate the subsequent ATP-dependent translocation. The ability to subdivide translocation into individual reactions provides a more precise means of determining the membrane components involved in this process.

摘要

我们使用了一种无细胞质的检测方法,当将亲和纯化的外膜蛋白A前体(proOmpA)从8 M尿素中稀释到酵母糙面微粒体悬液中时,可实现有效的转运和信号肽切割。蛋白质靶向和转运的这一方面发生在两个可区分的步骤中:(a)在没有ATP和细胞质因子的情况下,前体与膜结合但不发生转运;(b)添加ATP会导致结合的前体转运并加工成成熟形式。放射性标记的proOmpA与微粒体的结合是可饱和的,添加未标记的proOmpA可抑制这种结合,但成熟的OmpA或其他蛋白质则不能。放射性标记的前原α因子与其他前体蛋白也能有效竞争结合,但成熟蛋白则不能。Scatchard分析表明proOmpA的解离常数(Kd)为7.5×10^(-9) M。结合很可能是由蛋白质介导的,因为发现用蛋白酶木瓜蛋白酶处理微粒体会产生抑制作用。这些结果代表了分泌蛋白前体与膜结合的首次功能表征。用NEM对微粒体进行烷基化处理、用尿素洗涤膜或在非允许温度下使用(转运)突变体ptll的膜,均不影响结合,但确实消除了随后的ATP依赖性转运。将转运细分为单个反应的能力提供了一种更精确的方法来确定参与此过程的膜成分。

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Secretion in yeast: preprotein binding to a membrane receptor and ATP-dependent translocation are sequential and separable events in vitro.酵母中的分泌:前体蛋白与膜受体的结合以及ATP依赖性转运在体外是相继且可分离的事件。
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本文引用的文献

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Secretion in yeast: translocation and glycosylation of prepro-alpha-factor in vitro can occur via an ATP-dependent post-translational mechanism.酵母中的分泌:体外前原α因子的转运和糖基化可通过一种依赖ATP的翻译后机制发生。
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7
Trigger factor: a soluble protein that folds pro-OmpA into a membrane-assembly-competent form.触发因子:一种可溶性蛋白质,可将前OmpA折叠成具有膜组装能力的形式。
Proc Natl Acad Sci U S A. 1987 Aug;84(15):5216-20. doi: 10.1073/pnas.84.15.5216.
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70K heat shock related proteins stimulate protein translocation into microsomes.70K热休克相关蛋白刺激蛋白质转运至微粒体中。
Nature. 1988 Apr 28;332(6167):805-10. doi: 10.1038/332805a0.
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A subfamily of stress proteins facilitates translocation of secretory and mitochondrial precursor polypeptides.应激蛋白的一个亚家族促进分泌性和线粒体前体多肽的转运。
Nature. 1988 Apr 28;332(6167):800-5. doi: 10.1038/332800a0.
10
Protein unfolding and the energetics of protein translocation across biological membranes.蛋白质解折叠与蛋白质跨生物膜转运的能量学
Cell. 1988 Feb 26;52(4):481-3. doi: 10.1016/0092-8674(88)90458-8.