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骨吸收破骨细胞中V-ATP酶不同亚基的mRNA的再吸收周期依赖性极化。

Resorption-cycle-dependent polarization of mRNAs for different subunits of V-ATPase in bone-resorbing osteoclasts.

作者信息

Laitala-Leinonen T, Howell M L, Dean G E, Väänänen H K

机构信息

Department of Anatomy, University of Oulu, Finland.

出版信息

Mol Biol Cell. 1996 Jan;7(1):129-42. doi: 10.1091/mbc.7.1.129.

Abstract

Protein sorting in eukaryotic cells is mainly done by specific targeting of polypeptides. The present evidence from oocytes, neurons, and some other polarized cells suggests that protein sorting can be further facilitated by concentrating mRNAs to their corresponding subcellular areas. However, very little is known about the mechanism(s) involved in mRNA targeting, or how widespread and dynamic such mRNA sorting might be. In this study, we have used an in vitro cell culture system, where large multinucleated osteoclasts undergo continuous structural and functional changes from polarized (resorbing) to a nonpolarized (resting) stage. We demonstrate here, using a nonradioactive in situ hybridization technique and confocal microscopy, that mRNAs for several vacuolar H(+)-ATPase subunits change their localization and polarity in osteoclasts according to the resorption cycle, whereas mRNA for cytoplasmic carbonic anhydrase II is found diffusely located throughout the osteoclast during the whole resorption cycle. Antisense RNA against the 16-kDa or 60-kDa V-ATPase subunit inhibits polarization of the osteoclasts, as determined by cytoskeleton staining. Antisense RNA against carbonic anhydrase II, however, has no such effect.

摘要

真核细胞中的蛋白质分选主要通过多肽的特异性靶向来完成。目前来自卵母细胞、神经元和其他一些极化细胞的证据表明,通过将mRNA集中到其相应的亚细胞区域可以进一步促进蛋白质分选。然而,对于mRNA靶向所涉及的机制,或者这种mRNA分选的广泛程度和动态性知之甚少。在本研究中,我们使用了一种体外细胞培养系统,其中大型多核破骨细胞经历从极化(吸收)到非极化(静止)阶段的持续结构和功能变化。我们在此使用非放射性原位杂交技术和共聚焦显微镜证明,几种液泡H(+) -ATP酶亚基的mRNA在破骨细胞中根据吸收周期改变其定位和极性,而细胞质碳酸酐酶II的mRNA在整个吸收周期中分散地位于破骨细胞中。通过细胞骨架染色确定,针对16-kDa或60-kDa V-ATP酶亚基的反义RNA抑制破骨细胞的极化。然而,针对碳酸酐酶II的反义RNA没有这种作用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/dc18/278618/cccea3e96bb5/mbc00008-0136-a.jpg

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