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Immunocytochemical localization of a large intrinsic membrane protein to the incisures and margins of frog rod outer segment disks

机译:大型内在膜蛋白的免疫细胞化学定位到蛙杆外节盘的边缘和边缘

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摘要

Immunocytochemical techniques have localized a large protein which is an intrinsic membrane component of isolated frog rod outer segments (ROS). This large protein whose apparent mol wt is 290,000 daltons comprises about 1--3% of the ROS membrane mass. Its molar ratio to opsin is between 1:300 and 1:900. Adequate immune responses were obtained with less than 30 microgram (100 pmol) of antigen per rabbit. Antibodies to the large protein were used for its localization on thin sections of frog retina embedded in glutaraldehyde cross-linked bovine serum albumin (BSA). Specifically bound antibodies were detected by an indirect sequence with ferritin-conjugated antibodies. This technique detected the protein which is represented by 1,000--3,000 molecules per disk. This indicates that the procedure is sufficiently sensitive for analysis of membrane components in low molar proportions. The large protein was specifically localized to the incisures of ROS disks which divide the disks into lobes and to the disk margin. Thus, opsin is mobile within the membrane of the disk while the large protein is apparently constrained to the disk edges. This finding raises the possibility that special functions are also localized ot his unusual region of high curvature, and that collisions of bleached opsin with these edges are physiologically important in couter segment function.
机译:免疫细胞化学技术已经定位了一种大蛋白,该蛋白是分离的蛙杆外部节段(ROS)的固有膜成分。这种大分子的表观分子量为290,000道尔顿,约占ROS膜质量的1--3%。它与视蛋白的摩尔比为1:300至1:900。每只兔子用不到30微克(100 pmol)的抗原获得足够的免疫反应。针对大蛋白的抗体被用于定位在戊二醛交联的牛血清白蛋白(BSA)中嵌入的青蛙视网膜的薄片上。通过结合铁蛋白的抗体的间接序列检测特异性结合的抗体。这项技术检测到的蛋白质由每个磁盘1,000--3,000个分子表示。这表明该程序对于分析低摩尔比例的膜成分足够灵敏。大蛋白专门定位在ROS圆盘的切口处,后者将圆盘划分为裂片和圆盘边缘。因此,视蛋白在盘的膜内是可移动的,而大的蛋白质显然被限制在盘的边缘。这一发现增加了特殊功能也可能定位于其异常的高曲率区域的可能性,并且漂白视蛋白与这些边缘的碰撞在生理段功能中具有重要的生理意义。

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