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膀胱的管腔质膜。II. 膜成分的分离与结构

Lumenal plasma membrane of the urinary bladder. II. Isolation and structure of membrane components.

作者信息

Chlapowski F J, Bonneville M A, Staehelin L A

出版信息

J Cell Biol. 1972 Apr;53(1):92-104. doi: 10.1083/jcb.53.1.92.

Abstract

A technique has been devised for isolation of lumenal plasma membranes from transitional epithelial cells lining the urinary bladder in rabbits and for subsequent separation of particle-bearing plaque regions from particle-free areas of the membranes. The success of the procedures employed and their effects on the isolates were assessed by electron microscopy of conventional plastic sections, negatively stained preparations, and freeze-etch replicas. When bladders are distended with a solution of 0.01 M thioglycolic acid, which reduces sulfhydryl bridges, cytoplasmic filaments are disrupted, and large segments of the lumenal membranes rupture and float free into the lumen. A centrifugation procedure was developed for isolating a fraction enriched with the large fragments. A comparison of membranes isolated in the presence of thioglycolate with those isolated from epithelial cells homogenized in sucrose medium indicates that thioglycolate has little effect on their fine structure except for the removal of filaments which are normally associated with their cytoplasmic surface. The curved plaques of hexagonally arrayed particles and the particle-free interplaque regions, both characteristic of membranes before exposure to thioglycolate, are well preserved. Subsequent treatment of thioglycolate-isolated lumenal membranes with 1% sodium desoxycholate (DOC) severs many of the interplaque regions, releasing individual plaques in which the particles are more clearly visible than before exposure to desoxycholate. Presumably, DOC acts by disrupting the hydrophobic bonds within the membrane; therefore, this type of cohesive force probably is a major factor maintaining the structural integrity of interplaque regions. This conclusion is consistent with the observation that interplaque regions undergo freeze-cleaving like simple bilayers with a plane of hydrophobic bonding.

摘要

已设计出一种技术,用于从兔膀胱内衬的移行上皮细胞中分离管腔质膜,并随后从膜的无颗粒区域分离含颗粒的斑块区域。通过对常规塑料切片、负染制剂和冷冻蚀刻复制品进行电子显微镜检查,评估了所采用程序的成功与否及其对分离物的影响。当膀胱用0.01 M巯基乙酸溶液扩张时,该溶液会还原巯基桥,细胞质细丝被破坏,管腔膜的大片段破裂并游离到管腔中。开发了一种离心程序来分离富含大碎片的部分。将在巯基乙酸存在下分离的膜与在蔗糖培养基中匀浆的上皮细胞中分离的膜进行比较表明,巯基乙酸对其精细结构影响很小,只是去除了通常与其细胞质表面相关的细丝。六边形排列颗粒的弯曲斑块和无颗粒的斑块间区域,这两者都是暴露于巯基乙酸之前膜的特征,都保存完好。随后用1%脱氧胆酸钠(DOC)处理巯基乙酸分离的管腔膜,会切断许多斑块间区域,释放出单个斑块,其中颗粒比暴露于脱氧胆酸钠之前更清晰可见。据推测,DOC通过破坏膜内的疏水键起作用;因此,这种内聚力可能是维持斑块间区域结构完整性的主要因素。这一结论与斑块间区域像具有疏水键平面的简单双层一样经历冷冻断裂的观察结果一致。

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