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人类红细胞血影中带3蛋白与Triton壳的动态关联。

Dynamic association of band 3 with triton shells in human erythrocyte ghosts.

作者信息

Ueno E, Sato S, Jinbu Y, Nakao M

出版信息

Biochim Biophys Acta. 1987 Sep 2;915(1):77-86. doi: 10.1016/0167-4838(87)90127-0.

Abstract

To test a possibility that free band 3 and ankyrin-linked band 3 are exchanged in situ, band 3 was labeled with 125I, using intact red blood cells and lactoperoxidase. The cytoplasmic surface of this labeled band 3 was considered to be intact. When Triton shells were incubated with Triton supernatants prepared from 125I-labeled intact erythrocytes at 37 degrees C in the presence of Mg-ATP under isotonic conditions, the incorporation of free 125I-labeled band 3 to shells was observed. This incorporation was affected by the presence of Triton X-100 in the incubation mixture, and significantly decreased when the content of Triton X-100 was less than 0.04% (v/v). On the other hand, ankyrin-linked 125I-labeled band 3 was released when shells prepared from 125I-labeled intact erythrocytes were incubated with the Triton supernatants at 37 degrees C under the same condition as when free 125I-labeled band 3 incorporation was observed. These results strongly suggest that free and ankyrin-linked band 3 exchanged with each other in the presence of Triton X-100. A water-soluble 43 kDa fragment of band 3 inhibited the incorporation of free 125I-labeled band 3 to the shells and also inhibited the Mg-ATP-dependent shape change of ghosts in the absence of Triton X-100. Both of these inhibitory effects remained, even after 10 min of heat treatment at 100 degrees C, but drastically decreased by treatment with trypsin. Our results strongly suggest that a dynamic exchange of the free band 3 for ankyrin-linked band 3 may occur in intact erythrocytes, and it may even contribute to the shape change of erythrocytes.

摘要

为了测试游离带3和锚蛋白连接的带3在原位是否会发生交换,使用完整的红细胞和乳过氧化物酶,用125I标记带3。这种标记的带3的细胞质表面被认为是完整的。当在等渗条件下,在Mg-ATP存在的情况下,将Triton壳与从125I标记的完整红细胞制备的Triton上清液在37℃孵育时,观察到游离的125I标记的带3掺入到壳中。这种掺入受到孵育混合物中Triton X-100的存在的影响,当Triton X-100的含量小于0.04%(v/v)时,掺入显著减少。另一方面,当将从125I标记的完整红细胞制备的壳与Triton上清液在与观察到游离的125I标记的带3掺入时相同的条件下于37℃孵育时,锚蛋白连接的125I标记的带3会被释放出来。这些结果有力地表明,在Triton X-100存在的情况下,游离的和锚蛋白连接的带3会相互交换。带3的一种水溶性43 kDa片段抑制了游离的125I标记的带3掺入到壳中,并且在没有Triton X-100的情况下也抑制了Mg-ATP依赖性的血影形状变化。即使在100℃热处理10分钟后,这两种抑制作用仍然存在,但用胰蛋白酶处理后会急剧下降。我们的结果有力地表明,在完整的红细胞中可能会发生游离带3与锚蛋白连接的带3之间的动态交换,甚至可能有助于红细胞的形状变化。

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