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本文引用的文献

1
Acute internalization of gap junctions in vascular endothelial cells in response to inflammatory mediator-induced G-protein coupled receptor activation.血管内皮细胞中缝隙连接的急性内化,以响应炎症介质诱导的G蛋白偶联受体激活。
FEBS Lett. 2008 Dec 10;582(29):4039-46. doi: 10.1016/j.febslet.2008.10.043. Epub 2008 Nov 4.
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Double-membrane gap junction internalization requires the clathrin-mediated endocytic machinery.双膜间隙连接内化需要网格蛋白介导的内吞机制。
FEBS Lett. 2008 Aug 20;582(19):2887-92. doi: 10.1016/j.febslet.2008.07.024. Epub 2008 Jul 24.
3
Invasive and adherent bacterial pathogens co-Opt host clathrin for infection.侵袭性和黏附性细菌病原体共同利用宿主网格蛋白进行感染。
Cell Host Microbe. 2007 Nov 15;2(5):340-51. doi: 10.1016/j.chom.2007.10.001.
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Clathrin: an amazing multifunctional dreamcoat?网格蛋白:一件神奇的多功能“梦之衣”?
Cell Host Microbe. 2007 Nov 15;2(5):288-90. doi: 10.1016/j.chom.2007.10.007.
5
Connexin36 vs. connexin32, "miniature" neuronal gap junctions, and limited electrotonic coupling in rodent suprachiasmatic nucleus.连接蛋白36与连接蛋白32、“微型”神经元缝隙连接以及啮齿动物视交叉上核中有限的电紧张性耦合
Neuroscience. 2007 Oct 26;149(2):350-71. doi: 10.1016/j.neuroscience.2007.06.052. Epub 2007 Jul 21.
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Tracking intracellular protein movements using photoswitchable fluorescent proteins PS-CFP2 and Dendra2.使用光开关荧光蛋白PS-CFP2和Dendra2追踪细胞内蛋白质运动。
Nat Protoc. 2007;2(8):2024-32. doi: 10.1038/nprot.2007.291.
7
Microtubule plus-end-tracking proteins target gap junctions directly from the cell interior to adherens junctions.微管正端追踪蛋白直接从细胞内部将间隙连接靶向至黏着连接。
Cell. 2007 Feb 9;128(3):547-60. doi: 10.1016/j.cell.2006.12.037.
8
Internalization of large double-membrane intercellular vesicles by a clathrin-dependent endocytic process.通过网格蛋白依赖性内吞过程实现大的双膜细胞间囊泡的内化。
Mol Biol Cell. 2007 Feb;18(2):337-47. doi: 10.1091/mbc.e06-06-0487. Epub 2006 Nov 15.
9
Abundance and ultrastructural diversity of neuronal gap junctions in the OFF and ON sublaminae of the inner plexiform layer of rat and mouse retina.大鼠和小鼠视网膜内丛状层 OFF 和 ON 亚层中神经元缝隙连接的丰度和超微结构多样性
Neuroscience. 2006 Nov 3;142(4):1093-117. doi: 10.1016/j.neuroscience.2006.08.020. Epub 2006 Sep 28.
10
Engineering of a monomeric green-to-red photoactivatable fluorescent protein induced by blue light.蓝光诱导的单体绿色到红色光激活荧光蛋白的工程改造。
Nat Biotechnol. 2006 Apr;24(4):461-5. doi: 10.1038/nbt1191. Epub 2006 Mar 19.

间隙连接的更新是通过小的内吞双膜囊泡的内化来实现的。

Gap junction turnover is achieved by the internalization of small endocytic double-membrane vesicles.

作者信息

Falk Matthias M, Baker Susan M, Gumpert Anna M, Segretain Dominique, Buckheit Robert W

机构信息

Department of Biological Sciences, Lehigh University, Bethlehem, PA 18015, USA.

出版信息

Mol Biol Cell. 2009 Jul;20(14):3342-52. doi: 10.1091/mbc.e09-04-0288. Epub 2009 May 20.

DOI:10.1091/mbc.e09-04-0288
PMID:19458184
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2710821/
Abstract

Double-membrane-spanning gap junction (GJ) channels cluster into two-dimensional arrays, termed plaques, to provide direct cell-to-cell communication. GJ plaques often contain circular, channel-free domains ( approximately 0.05-0.5 mum in diameter) identified >30 y ago and termed nonjunctional membrane (NM) domains. We show, by expressing the GJ protein connexin43 (Cx43) tagged with green fluorescent protein, or the novel photoconvertible fluorescent protein Dendra2, that NM domains appear to be remnants generated by the internalization of small GJ channel clusters that bud over time from central plaque areas. Channel clusters internalized within seconds forming endocytic double-membrane GJ vesicles ( approximately 0.18-0.27 mum in diameter) that were degraded by lysosomal pathways. Surprisingly, NM domains were not repopulated by surrounding channels and instead remained mobile, fused with each other, and were expelled at plaque edges. Quantification of internalized, photoconverted Cx43-Dendra2 vesicles indicated a GJ half-life of 2.6 h that falls within the estimated half-life of 1-5 h reported for GJs. Together with previous publications that revealed continuous accrual of newly synthesized channels along plaque edges and simultaneous removal of channels from plaque centers, our data suggest how the known dynamic channel replenishment of functional GJ plaques can be achieved. Our observations may have implications for the process of endocytic vesicle budding in general.

摘要

双膜跨越间隙连接(GJ)通道聚集成二维阵列,称为斑块,以提供细胞间的直接通讯。GJ斑块通常包含圆形的、无通道结构域(直径约0.05 - 0.5微米),这些结构域在30多年前就已被发现,被称为非连接膜(NM)结构域。我们通过表达标记有绿色荧光蛋白的GJ蛋白连接蛋白43(Cx43)或新型光转化荧光蛋白Dendra2发现,NM结构域似乎是小GJ通道簇内化产生的残余物,这些小通道簇随着时间的推移从中央斑块区域萌芽。通道簇在数秒内内化形成内吞性双膜GJ囊泡(直径约0.18 - 0.27微米),并通过溶酶体途径降解。令人惊讶的是,NM结构域没有被周围的通道重新填充,而是保持移动性,相互融合,并在斑块边缘被排出。对内化的、光转化的Cx43 - Dendra2囊泡的定量分析表明,GJ的半衰期为2.6小时,这与报道的GJ估计半衰期1 - 5小时相符。结合之前揭示新合成通道沿斑块边缘持续积累以及同时从斑块中心去除通道的出版物,我们的数据表明了功能性GJ斑块已知的动态通道补充是如何实现的。我们的观察结果可能对一般内吞囊泡萌芽过程有影响。