海胆卵中兰尼碱受体的检测及功能特性研究

Detection and functional characterization of ryanodine receptors from sea urchin eggs.

作者信息

Lokuta A J, Darszon A, Beltrán C, Valdivia H H

机构信息

Department of Physiology, University of Wisconsin Medical School, Madison, WI 53706, USA.

出版信息

J Physiol. 1998 Jul 1;510 ( Pt 1)(Pt 1):155-64. doi: 10.1111/j.1469-7793.1998.155bz.x.

DOI:10.1111/j.1469-7793.1998.155bz.x

PMID:9625874

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2231031/

Abstract

Immunoblot analysis, [3H]ryanodine binding, and planar lipid bilayer techniques were used to identify and characterize the functional properties of ryanodine receptors (RyRs) from Lytechinus pictus and Strongylocentrotus purpuratus sea urchin eggs. 2. An antibody against mammalian skeletal RyRs identified an approximately 400 kDa band in the cortical microsomes of sea urchin eggs while a cardiac-specific RyR antibody failed to recognize this protein. [3H]Ryanodine binding to cortical microsomes revealed the presence of a high-affinity (Kd = 13 nM), saturable (maximal density of receptor sites, Bmax = 1.56 pmol (mg protein)-1) binding site that exhibited a biphasic response to Ca2+. 3. Upon reconstitution of cortical microsomes into lipid bilayers, only sparse and unstable openings of a high-conductance cation channel were detected. Addition of crude sea urchin egg homogenate to the cytosolic (cis side) of the channel increased the frequency of openings and stabilized channel activity. The homogenate-activated channels were Ca2+ sensitive, selective for Ca2+ over Cs+, and driven by ryanodine into a long-lived subconductance state that represented approximately 40 % of the full conductance level. Homogenate dialysed in membranes with a molecular weight cut-off <= 2000 lacked the capacity to increase the frequency of RyR openings and to stabilize channel activity. 4. Direct application of cyclic adenosine diphosphoribose (cADPR) or photolysis of NPE-cADPR ('caged' cADPR) by ultraviolet laser pulses produced transient activation of sea urchin egg RyRs. Calmodulin (CaM) failed to activate reconstituted RyRs; however, channel activity was inhibited by the CaM blocker trifluoroperazine, suggesting that CaM was necessary but not sufficient to sustain RyR activity. 5. These findings suggest that a functional Ca2+ release unit in sea urchin eggs is a complex of several molecules, one of which corresponds to a protein functionally similar to mammalian RyRs.

摘要

采用免疫印迹分析、[3H]ryanodine结合以及平面脂质双层技术来鉴定和表征来自花斑海胆（Lytechinus pictus）和紫球海胆（Strongylocentrotus purpuratus）卵的ryanodine受体（RyRs）的功能特性。2. 一种针对哺乳动物骨骼肌RyRs的抗体在海胆卵的皮质微粒体中鉴定出一条约400 kDa的条带，而一种心脏特异性RyR抗体未能识别该蛋白。[3H]ryanodine与皮质微粒体的结合揭示存在一个高亲和力（Kd = 13 nM）、可饱和（受体位点的最大密度，Bmax = 1.56 pmol（mg蛋白）-1）的结合位点，该位点对Ca2+表现出双相反应。3. 将皮质微粒体重构成脂质双层后，仅检测到高电导阳离子通道的稀疏且不稳定的开放。向通道的胞质（顺式侧）添加粗制海胆卵匀浆增加了开放频率并稳定了通道活性。匀浆激活的通道对Ca2+敏感，对Ca2+的选择性高于Cs+，并被ryanodine驱动进入代表约40%全电导水平的长寿命亚电导状态。在分子量截留值<= 2000的膜中透析的匀浆缺乏增加RyR开放频率和稳定通道活性的能力。4. 直接应用环腺苷二磷酸核糖（cADPR）或通过紫外激光脉冲光解NPE - cADPR（“笼化”cADPR）可使海胆卵RyRs产生瞬时激活。钙调蛋白（CaM）未能激活重构的RyRs；然而，通道活性被CaM阻滞剂三氟拉嗪抑制，这表明CaM对于维持RyR活性是必要但不充分的。5. 这些发现表明海胆卵中的功能性Ca2+释放单位是几种分子的复合物，其中之一对应于一种在功能上与哺乳动物RyRs相似的蛋白质。