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本文引用的文献

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Analysis of the neural crest ventral pathway using injected tracer cells.使用注射示踪细胞对神经嵴腹侧通路进行分析。
Dev Biol. 1980 Jun 1;77(1):130-41. doi: 10.1016/0012-1606(80)90461-3.
2
Pathways and mechanisms of avian trunk neural crest cell migration and localization.禽类躯干神经嵴细胞迁移和定位的途径与机制。
Dev Biol. 1982 Oct;93(2):324-43. doi: 10.1016/0012-1606(82)90121-x.
3
Distribution of fibronectin in the early phase of avian cephalic neural crest cell migration.纤连蛋白在禽类头部神经嵴细胞迁移早期阶段的分布
Dev Biol. 1982 Oct;93(2):308-23. doi: 10.1016/0012-1606(82)90120-8.
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Monoclonal antibodies which alter the morphology of cultured chick myogenic cells.可改变培养鸡成肌细胞形态的单克隆抗体。
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Immunocytochemical localization of fibronectin in embryonic chick trunk and area vasculosa.纤连蛋白在鸡胚躯干和血管区的免疫细胞化学定位
Dev Biol. 1981 Mar;82(2):267-86. doi: 10.1016/0012-1606(81)90451-6.
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Fibronectin in early avian embryos: synthesis and distribution along the migration pathways of neural crest cells.早期鸟类胚胎中的纤连蛋白:沿神经嵴细胞迁移途径的合成与分布
Cell Tissue Res. 1980;211(2):269-91. doi: 10.1007/BF00236449.
7
Neural crest cell migration: requirements for exogenous fibronectin and high cell density.神经嵴细胞迁移:对外源纤连蛋白和高细胞密度的需求
J Cell Biol. 1983 Feb;96(2):462-73. doi: 10.1083/jcb.96.2.462.
8
New surface component of fibroblast's focal contacts identified by a monoclonal antibody.通过单克隆抗体鉴定出的成纤维细胞粘着斑新表面成分。
Cell. 1982 Dec;31(3 Pt 2):671-9. doi: 10.1016/0092-8674(82)90322-1.
9
Dualistic nature of adhesive protein function: fibronectin and its biologically active peptide fragments can autoinhibit fibronectin function.黏附蛋白功能的二元性:纤连蛋白及其生物活性肽片段可自动抑制纤连蛋白功能。
J Cell Biol. 1984 Jul;99(1 Pt 1):29-36. doi: 10.1083/jcb.99.1.29.
10
Spreading of explants of embryonic chick mesenchymes and epithelia on fibronectin and laminin.鸡胚间充质和上皮外植体在纤连蛋白和层粘连蛋白上的铺展。
Cell Tissue Res. 1984;236(2):265-77. doi: 10.1007/BF00214227.

一种影响细胞黏附的单克隆抗体对神经嵴迁移的改变。

Alterations in neural crest migration by a monoclonal antibody that affects cell adhesion.

作者信息

Bronner-Fraser M

出版信息

J Cell Biol. 1985 Aug;101(2):610-7. doi: 10.1083/jcb.101.2.610.

DOI:10.1083/jcb.101.2.610
PMID:4019585
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2113653/
Abstract

The possible role of a 140-kD cell surface complex in neural crest adhesion and migration was examined using a monoclonal antibody JG22, first described by Greve and Gottlieb (1982, J. Cell. Biochem. 18:221-229). The addition of JG22 to neural crest cells in vitro caused a rapid change in morphology of cells plated on either fibronectin or laminin substrates. The cells became round and phase bright, often detaching from the dish or forming aggregates of rounded cells. Other tissues such as somites, notochords, and neural tubes were unaffected by the antibody in vitro even though the JG22 antigen is detectable in embryonic tissue sections on the surface of the myotome, neural tube, and notochord. The effects of the JG22 on neural crest migration in vivo were examined by a new perturbation approach in which both the antibody and the hybridoma cells were microinjected onto neural crest pathways. Hybridoma cells were labeled with a fluorescent cell marker that is nondeleterious and that is preserved after fixation and tissue sectioning. The JG22 antibody and hybridoma cells caused a marked reduction in cranial neural crest migration, a build-up of neural crest cells within the lumen of the neural tube, and some migration along aberrant pathways. Neural crest migration in the trunk was affected to a much lesser extent. In both cranial and trunk regions, a cell free zone of one or more cell diameters was generally observed between neural crest cells and the JG22 hybridoma cells. Two other monoclonal antibodies, 1-B and 1-N, were used as controls. Both 1-B and 1-N bind to bands of the 140-kD complex precipitated by JG22. Neither control antibody affected neural crest adhesion in vitro or neural crest migration in situ. This suggests that the observed alterations in neural crest migration are due to a functional block of the 140-kD complex.

摘要

利用单克隆抗体JG22研究了140-kD细胞表面复合物在神经嵴黏附与迁移中的可能作用,该抗体最早由Greve和Gottlieb于1982年报道(《细胞生物化学杂志》18:221 - 229)。在体外将JG22添加到神经嵴细胞中,会使接种在纤连蛋白或层粘连蛋白底物上的细胞形态迅速改变。细胞会变圆且折光性增强,常常从培养皿上脱离或形成圆形细胞聚集体。其他组织如体节、脊索和神经管在体外不受该抗体影响,尽管在胚胎组织切片中,肌节、神经管和脊索表面可检测到JG22抗原。通过一种新的干扰方法研究了JG22对体内神经嵴迁移的影响,即将抗体和杂交瘤细胞都微量注射到神经嵴路径上。杂交瘤细胞用一种无害的荧光细胞标记物标记,该标记物在固定和组织切片后仍能保留。JG22抗体和杂交瘤细胞导致颅神经嵴迁移显著减少,神经嵴细胞在神经管腔内积聚,并出现一些沿异常路径的迁移。躯干神经嵴迁移受影响程度小得多。在颅部和躯干区域,通常在神经嵴细胞与JG22杂交瘤细胞之间观察到一个或多个细胞直径的无细胞区。另外两种单克隆抗体1 - B和1 - N用作对照。1 - B和1 - N都与JG22沉淀的140-kD复合物条带结合。两种对照抗体在体外均不影响神经嵴黏附,在原位也不影响神经嵴迁移。这表明观察到的神经嵴迁移改变是由于140-kD复合物的功能阻断所致。