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转基因 GDNF 前体和前肽区域的可用性影响诱导轴突芽生长的能力。

Availability of Pre- and Pro-regions of Transgenic GDNF Affects the Ability to Induce Axonal Sprout Growth.

机构信息

Institute of Gene Biology, Russian Academy of Sciences, 34 Vavilov St., 119334, Moscow, Russia.

出版信息

Mol Neurobiol. 2015;51(3):1195-205. doi: 10.1007/s12035-014-8792-8. Epub 2014 Jul 3.

Abstract

Plasmids containing four GFP-tagged isoforms of the human GDNF gene, with both pre- and pro-regions (pre-pro- GDNF), with the pre- (pre-GDNF) or the pro-region (pro-GDNF) alone, and without the pre- and pro-regions (mGDNF), were used to transfect HEK293 cells (human embryonic kidney cell line). The effect of the transgenic products on the growth of processes was studied in the spinal ganglia of 14-day rat embryos. Media conditioned by the transgenic cells were used to culture explants and dissociated cells of embryonic dorsal root ganglia attached to the bottom of the plate. Medium conditioned by gfp-transgenic HEK293 cells was used as the control. Spinal ganglia explants and dissociated cells cultured in a medium supplemented with recombinant GDNF (recGDNF) as well as in conditioned media containing the pre-GDNF and mGDNF products demonstrated active growth of processes immunopositive for neuronal marker beta-3-tubulin as early as on culture day 4. The ganglia and cells cultured in control medium and media conditioned by cells transgenic for pro-GDNF had no or very few processes even after 10 days of culture.

摘要

使用含有人类 GDNF 基因的四个 GFP 标记同工型的质粒,带有前导和前肽区(前-前肽-GDNF),只有前导区(前-GDNF)或前肽区(前肽-GDNF),没有前导和前肽区(mGDNF),转染 HEK293 细胞(人胚肾细胞系)。研究了转基因产物对 14 天大鼠胚胎脊髓神经节中突起生长的影响。用转基因细胞的条件培养基培养贴附在平板底部的胚胎背根神经节的外植体和分离细胞。用 GFP 转基因 HEK293 细胞的条件培养基作为对照。在添加重组 GDNF(recGDNF)的培养基中培养的脊髓神经节外植体和分离细胞,以及含有前-GDNF 和 mGDNF 产物的条件培养基中培养的细胞,在培养第 4 天就表现出神经元标记物 beta-3-微管蛋白免疫阳性的突起的活跃生长。在对照培养基和转导 pro-GDNF 的细胞的条件培养基中培养的神经节和细胞,即使在培养 10 天后,也没有或只有很少的突起。

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