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毛细胞静纤毛的“束状印迹”纯化及蛋白质初步表征

"Bundle blot" purification and initial protein characterization of hair cell stereocilia.

作者信息

Shepherd G M, Barres B A, Corey D P

机构信息

Howard Hughes Medical Institute, Massachusetts General Hospital, Boston 02114.

出版信息

Proc Natl Acad Sci U S A. 1989 Jul;86(13):4973-7. doi: 10.1073/pnas.86.13.4973.

Abstract

Stereocilia were isolated from bullfrog (Rana catesbeiana) saccular hair cells by nitrocellulose adhesion. The high purity and high yield of the preparation were demonstrated by microscopy. SDS/PAGE of stereociliary proteins resolved 12-15 major bands. Actin, previously identified as a component of the stereociliary core, was identified in purified stereocilia as a band comigrating with authentic actin and by phalloidin labeling of intact isolated stereocilia. Fimbrin was identified in immunoblots of purified stereocilia. The most abundant other proteins migrated at 11, 14, 16-19, 27, and 36 kDa. Demembranated stereociliary cores consisted primarily of protein bands corresponding to actin and fimbrin and several proteins ranging from 43 to 63 kDa. Because the adaptation mechanism in hair cells is calcium-sensitive and seems localized to stereocilia, we sought evidence for calcium-binding proteins in stereocilia. Calmodulin and calbindin antibodies labeled stereocilia in intact cells. A protein band in purified stereocilia exhibited a Ca2+-dependent shift in electrophoretic mobility identical to that of authentic calmodulin, and the 27-kDa band may represent calbindin. These biochemical data demonstrate that stereocilia consist of a relatively small set of proteins. Most of these, including those involved in transduction and adaptation, are as yet uncharacterized. The availability of purified stereocilia should prove useful in further studies of structure-function relationships in these mechanically sensitive organelles.

摘要

通过硝酸纤维素黏附法从牛蛙(北美牛蛙)球囊毛细胞中分离出静纤毛。显微镜检查证明了该制剂的高纯度和高产量。静纤毛蛋白的SDS/PAGE分离出12 - 15条主要条带。肌动蛋白先前被鉴定为静纤毛核心的组成成分,在纯化的静纤毛中通过与真实肌动蛋白共迁移的条带以及对完整分离静纤毛的鬼笔环肽标记得以鉴定。在纯化静纤毛的免疫印迹中鉴定出丝束蛋白。其他最丰富的蛋白质在11、14、16 - 19、27和36 kDa处迁移。去膜静纤毛核心主要由对应于肌动蛋白和丝束蛋白的蛋白条带以及几种43至63 kDa的蛋白质组成。由于毛细胞中的适应机制对钙敏感且似乎定位于静纤毛,我们寻找静纤毛中钙结合蛋白的证据。钙调蛋白和钙结合蛋白抗体标记完整细胞中的静纤毛。纯化静纤毛中的一条蛋白条带在电泳迁移率上表现出与真实钙调蛋白相同的Ca2 +依赖性变化,并且27 kDa条带可能代表钙结合蛋白。这些生化数据表明静纤毛由相对较少的一组蛋白质组成。其中大多数,包括那些参与转导和适应的蛋白质,尚未得到表征。纯化静纤毛的可得性应证明对进一步研究这些机械敏感细胞器的结构 - 功能关系有用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/9872/297538/18ca38e9dc6c/pnas00280-0180-a.jpg

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