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植物细胞中不依赖钙离子和由钙离子/鸟苷三磷酸结合蛋白控制的胞吐作用。

Ca2+-independent and Ca2+/GTP-binding protein-controlled exocytosis in a plant cell.

作者信息

Homann U, Tester M

机构信息

Department of Plant Sciences, University of Cambridge, Downing Street, Cambridge CB2 3EA, United Kingdom.

出版信息

Proc Natl Acad Sci U S A. 1997 Jun 10;94(12):6565-70. doi: 10.1073/pnas.94.12.6565.

DOI:10.1073/pnas.94.12.6565
PMID:11038550
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC21090/
Abstract

Exocytosis allows the release of secretory products and the delivery of new membrane material to the plasma membrane. So far, little is known about the underlying molecular mechanism and its control in plant cells. We have used the whole-cell patch-clamp technique to monitor changes in membrane capacitance to study exocytosis in barley aleurone protoplasts. To investigate the involvement of Ca2+ and GTP-binding proteins in exocytosis, protoplasts were dialyzed with very low (<2 nM) and high (1 microM) free Ca2+ and nonhydrolyzable guanine nucleotides guanosine 5'-gamma-thio]triphosphate (GTP[gammaS]) or guanosine 5'-[beta-thio]diphosphate (GDP[betaS]). With less than 2 nM cytoplasmic free Ca2+, the membrane capacitance increased significantly over 20 min. This increase was not altered by GTP[gammaS] or GDP[betaS]. In contrast, dialyzing protoplasts with 1 microM free Ca2+ resulted in a large increase in membrane capacitance that was slightly reduced by GTP[gammaS] and strongly inhibited by GDP[betaS]. We conclude that two exocytotic pathways exist in barley aleurone protoplasts: one that is Ca2+-independent and whose regulation is currently not known and another that is stimulated by Ca2+ and modulated by GTP-binding proteins. We suggest that Ca2+-independent exocytosis may be involved in cell expansion in developing protoplasts. Ca2+-stimulated exocytosis may play a role in gibberellic acid-stimulated alpha-amylase secretion in barley aleurone and, more generally, may be involved in membrane resealing in response to cell damage.

摘要

胞吐作用允许分泌产物的释放以及新的膜材料输送到质膜。到目前为止,关于植物细胞中潜在的分子机制及其调控知之甚少。我们使用全细胞膜片钳技术监测膜电容的变化,以研究大麦糊粉层原生质体中的胞吐作用。为了研究Ca2+和GTP结合蛋白在胞吐作用中的作用,用极低(<2 nM)和高(1 microM)游离Ca2+以及不可水解的鸟嘌呤核苷酸鸟苷5'-γ-硫代三磷酸(GTP[γS])或鸟苷5'-β-硫代二磷酸(GDP[βS])对原生质体进行透析。当细胞质游离Ca2+低于2 nM时,膜电容在20分钟内显著增加。这种增加不受GTP[γS]或GDP[βS]的影响。相反,用1 microM游离Ca2+透析原生质体会导致膜电容大幅增加,GTP[γS]使其略有降低,而GDP[βS]则强烈抑制。我们得出结论,大麦糊粉层原生质体中存在两条胞吐途径:一条是Ca2+非依赖性的,其调控目前尚不清楚;另一条是由Ca2+刺激并受GTP结合蛋白调节的。我们认为Ca2+非依赖性胞吐作用可能参与发育中的原生质体的细胞扩张。Ca2+刺激的胞吐作用可能在大麦糊粉层中赤霉素刺激的α-淀粉酶分泌中起作用,更普遍地说,可能参与对细胞损伤的膜重新封闭。

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