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从早期海鞘胚胎分离的卵裂阻滞卵裂球中诱导神经型分化。

Induced neural-type differentiation in the cleavage-arrested blastomere isolated from early ascidian embryos.

作者信息

Okado H, Takahashi K

机构信息

Department of Neurobiology, Faculty of Medicine, University of Tokyo, Japan.

出版信息

J Physiol. 1990 Aug;427:603-23. doi: 10.1113/jphysiol.1990.sp018190.

DOI:10.1113/jphysiol.1990.sp018190
PMID:2213609
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1189949/
Abstract
  1. Isolated blastomeres and pairs of blastomeres from 8-cell embryos of Halocynthia roretzi and Halocynthia aurantium were cleavage-arrested with cytochalasin B and cultured. Their differentiation was examined in terms of membrane excitability, immunoreactivity to an epidermis-specific monoclonal antibody (2C5), and the presence of acetylcholinesterase. 2. The blastomeres that showed epidermal-type differentiation had Ca2(+)-dependent action potentials and membrane currents, and immunoreactivity to 2C5. The blastomeres that showed neural-type differentiation had Na(+)-, Ca2(+)- and TEA-sensitive delayed K+ channels, and lacked immunoreactivity to 2C5. 3. Cleavage-arrested anterior-animal blastomeres, a4-2, when cultured in isolation from an 8-cell embryo, differentiated exclusively into epidermal-type cells. However, when cultured in contact with anterior-vegetal blastomeres, A4-1, they mostly showed neural-type differentiation (seventeen out of twenty-four cells in H. roretzi). 4. Reduction of the cytochalasin B concentration enhanced neural-type development of a4-2 blastomeres in contact with A4-1 blastomeres in H. aurantium, possibly by tightening the physical contact between the blastomeres. 5. When a cleavage-arrested and isolated a4-2 blastomere was treated with 2% pronase at 10 degrees C for 15 min at the time when sister control embryos reached the 32-cell stage, the blastomere underwent neural-type differentiation in a manner identical to that of a4-2 blastomeres contacted by A4-1 cells. 6. The period during which neural-type differentiation of a4-2 blastomeres could be induced by treatment with pronase was from the 8-cell to the 110-cell stage. At the late gastrula stage neural-type differentiation of a4-2 blastomeres was not induced by pronase. The effective period for neural-type differentiation of a4-2 blastomeres in contact with A4-1 cells was between the 64-cell stage and late gastrula stage. Competence of the a4-2 blastomere to undergo neural-type differentiation decreased during gastrula stages, while the inducing ability of the A4-1 blastomere lasted longer. 7. In a few cases the posterior-animal blastomere, b4-2, could also be induced to undergo neural-type differentiation after contact with A4-1 cells or after pronase treatment. 8. The appearance of Na+ spikes in a4-2 blastomeres in contact with A4-1 cells was considered a manifestation of neural induction, similar in principle to the induction of ectoderm by the chorda-mesoderm in higher vertebrates.
摘要
  1. 用细胞松弛素B使罗氏海鞘和金色海鞘8细胞胚胎的单个卵裂球及卵裂球对停止分裂并进行培养。从膜兴奋性、对表皮特异性单克隆抗体(2C5)的免疫反应性以及乙酰胆碱酯酶的存在情况方面检测它们的分化。2. 表现出表皮型分化的卵裂球具有Ca2(+)依赖性动作电位和膜电流,以及对2C5的免疫反应性。表现出神经型分化的卵裂球具有Na(+)、Ca2(+)和TEA敏感的延迟K+通道,并且缺乏对2C5的免疫反应性。3. 从8细胞胚胎中分离培养的卵裂球停止分裂的前动物极卵裂球a4 - 2仅分化为表皮型细胞。然而,当与前植物极卵裂球A4 - 1接触培养时,它们大多表现出神经型分化(罗氏海鞘中24个细胞中有17个)。4. 降低细胞松弛素B的浓度增强了金色海鞘中与A4 - 1卵裂球接触的a4 - 2卵裂球的神经型发育,这可能是通过加强卵裂球之间的物理接触实现的。5. 当姐妹对照胚胎达到32细胞期时,将停止分裂并分离的a4 - 2卵裂球在10℃用2%链霉蛋白酶处理15分钟,该卵裂球以与被A4 - 1细胞接触的a4 - 2卵裂球相同的方式进行神经型分化。6. 用链霉蛋白酶处理可诱导a4 - 2卵裂球进行神经型分化的时期是从8细胞期到110细胞期。在原肠胚后期,链霉蛋白酶不能诱导a4 - 2卵裂球进行神经型分化。与A4 - 1细胞接触的a4 - 2卵裂球进行神经型分化的有效期是在64细胞期到原肠胚后期之间。a4 - 2卵裂球进行神经型分化的能力在原肠胚期降低,而A4 - 1卵裂球的诱导能力持续时间更长。7. 在少数情况下,后动物极卵裂球b4 - 2在与A4 - 1细胞接触或经链霉蛋白酶处理后也可被诱导进行神经型分化。8. 与A4 - 1细胞接触的a4 - 2卵裂球中Na+尖峰的出现被认为是神经诱导的一种表现,其原理类似于高等脊椎动物中脊索中胚层对外胚层的诱导。
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/83b0/1189949/e63264568bf8/jphysiol00461-0606-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/83b0/1189949/e63264568bf8/jphysiol00461-0606-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/83b0/1189949/e63264568bf8/jphysiol00461-0606-a.jpg

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本文引用的文献

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Further investigations of the differentiation in vitro of presumptive epidermis cells of the Rana pipiens gastrula.对豹蛙原肠胚假定表皮细胞体外分化的进一步研究。
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碱性成纤维细胞生长因子对海鞘外胚层卵裂球中神经元离子通道表达的诱导作用
J Physiol. 1998 Sep 1;511 ( Pt 2)(Pt 2):347-59. doi: 10.1111/j.1469-7793.1998.347bh.x.
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Neuronal expression in cleavage-arrested ascidian blastomeres requires gap junctional uncoupling from neighbouring cells.在卵裂停滞的海鞘卵裂球中的神经元表达需要与相邻细胞的间隙连接解偶联。
J Physiol. 1996 Mar 15;491 ( Pt 3)(Pt 3):825-42. doi: 10.1113/jphysiol.1996.sp021260.
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Neural differentiation in cleavage-arrested ascidian blastomeres induced by a proteolytic enzyme.蛋白水解酶诱导卵裂阻滞的海鞘卵裂球发生神经分化。
J Physiol. 1993 Apr;463:269-90. doi: 10.1113/jphysiol.1993.sp019594.
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Neural induction suppresses early expression of the inward-rectifier K+ channel in the ascidian blastomere.神经诱导抑制海鞘卵裂球中内向整流钾通道的早期表达。
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Differentiation of membrane excitability in isolated cleavage-arrested blastomeres from early ascidian embryos.早期海鞘胚胎中分离出的卵裂阻滞的卵裂球的膜兴奋性分化
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Inactivation kinetics of the sodium channel in the egg and the isolated, neurally differentiated blastomere of the ascidian.海鞘卵及分离的、神经分化的卵裂球中钠通道的失活动力学
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Cell lineage analysis of neural induction: origins of cells forming the induced nervous system.神经诱导的细胞谱系分析:形成诱导神经系统的细胞起源
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A simple "neural induction" model with two interacting cleavage-arrested ascidian blastomeres.一个具有两个相互作用的卵裂停滞海鞘卵裂球的简单“神经诱导”模型。
Proc Natl Acad Sci U S A. 1988 Aug;85(16):6197-201. doi: 10.1073/pnas.85.16.6197.