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Rap2 在 T 细胞迁移过程中循环利用 LFA-1 延伸构象中的作用。

A role for Rap2 in recycling the extended conformation of LFA-1 during T cell migration.

机构信息

Leukocyte Adhesion Laboratory, Cancer Research UK, London Research Institute London EC1V 4AD , UK.

出版信息

Biol Open. 2012 Nov 15;1(11):1161-8. doi: 10.1242/bio.20122824. Epub 2012 Sep 20.

DOI:10.1242/bio.20122824
PMID:23213397
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3507183/
Abstract

T lymphocytes make use of their major integrin LFA-1 to migrate on surfaces that express ICAM-1 such as blood vessels and inflamed tissue sites. How the adhesions are turned over in order to supply traction for this migration has not been extensively investigated. By following the fate of biotinylated membrane LFA-1 on T lymphocytes, we show in this study that LFA-1 internalization and re-exposure on the plasma membrane are linked to migration. Previously we demonstrated the GTPase Rap2 to be a regulator of LFA-1-mediated migration. SiRNA knockdown of this GTPase inhibits both LFA-1 internalization and also its ability to be re-exposed, indicating that Rap2 participates in recycling of LFA-1 and influences its complete endocytosis-exocytosis cycle. Confocal microscopy images reveal that the intracellular distribution of Rap2 overlaps with endosomal recycling vesicles. Although the homologous GTPase Rap1 is also found on intracellular vesicles and associated with LFA-1 activation, these two homologous GTPases do not co-localize. Little is known about the conformation of the LFA-1 that is recycled. We show that the extended form of LFA-1 is internalized and in Rap2 siRNA-treated T lymphocytes the trafficking of this LFA-1 conformation is disrupted resulting in its intracellular accumulation. Thus LFA-1-mediated migration of T lymphocytes requires Rap2-expressing vesicles to recycle the extended form of LFA-1 that we have previously found to control migration at the leading edge.

摘要

T 淋巴细胞利用其主要整合素 LFA-1 在表达 ICAM-1 的表面上迁移,例如血管和炎症组织部位。为了提供这种迁移的牵引力,粘附物是如何翻转的还没有被广泛研究。通过跟踪生物素化膜 LFA-1 在 T 淋巴细胞上的命运,我们在本研究中表明,LFA-1 的内化和再暴露于质膜与迁移有关。先前我们证明 GTP 酶 Rap2 是 LFA-1 介导的迁移的调节剂。该 GTP 酶的 siRNA 敲低不仅抑制了 LFA-1 的内化,也抑制了其再暴露的能力,表明 Rap2 参与了 LFA-1 的回收,并影响其完整的内吞-胞吐循环。共聚焦显微镜图像显示,Rap2 的细胞内分布与内体回收小泡重叠。尽管同源 GTP 酶 Rap1 也存在于细胞内小泡上,并与 LFA-1 激活有关,但这两种同源 GTP 酶并不共定位。关于回收的 LFA-1 的构象知之甚少。我们表明,LFA-1 的延伸形式被内化,并且在 Rap2 siRNA 处理的 T 淋巴细胞中,这种 LFA-1 构象的运输被破坏,导致其在细胞内积累。因此,T 淋巴细胞的 LFA-1 介导的迁移需要表达 Rap2 的囊泡来回收我们之前发现控制前沿迁移的延伸形式的 LFA-1。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1c70/3507183/860545ee9bdf/bio-01-11-1161-f04.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1c70/3507183/8bb5f7ce2ebb/bio-01-11-1161-f01.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1c70/3507183/5ecfa7158fcb/bio-01-11-1161-f02.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1c70/3507183/31068616e288/bio-01-11-1161-f03.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1c70/3507183/860545ee9bdf/bio-01-11-1161-f04.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1c70/3507183/8bb5f7ce2ebb/bio-01-11-1161-f01.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1c70/3507183/5ecfa7158fcb/bio-01-11-1161-f02.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1c70/3507183/31068616e288/bio-01-11-1161-f03.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1c70/3507183/860545ee9bdf/bio-01-11-1161-f04.jpg

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