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糖酵解代谢在磷酸盐对大鼠二细胞胚胎发育抑制中的作用

Involvement of glycolytic metabolism in developmental inhibition of rat two-cell embryos by phosphate.

作者信息

Nishikimi A, Uekawa N, Yamada M

机构信息

Division of Applied Biosciences, Graduate School of Agriculture, Kyoto University, Japan.

出版信息

J Exp Zool. 2000 Dec 1;287(7):503-9. doi: 10.1002/1097-010x(20001201)287:7<503::aid-jez6>3.0.co;2-b.

Abstract

To elucidate the mechanism by which phosphate induces developmental inhibition of rat 2-cell embryos, we examined the mutual effects of glucose and other glycolytic and non-glycolytic sugars, the non-metabolizable glucose analogue, and glycolytic inhibitors on the inhibitory effect of phosphate. In the absence of glucose, 30-49% of embryos treated with 10-500 microM phosphate were able to develop to morula and blastocysts. On the other hand, in the presence of 5 mM glucose, 10 microM phosphate decreased the developmental rate of 2-cell embryos to the 4-cell stage and completely inhibited the development beyond the 4-cell stage. In contrast, glucose showed no influence on development in phosphate-free medium. Similarly to glucose, the other glycolytic sugars fructose (5 mM) and mannose (5 mM) enhanced the inhibitory effect of 10 microM phosphate but had no influence in the absence of phosphate. In contrast, the non-glycolytic sugar and non-metabolizable glucose analogue N-acetylglucosamine and 3-O-methylglucose (3-O-MGlc), respectively, did not enhance the effects of phosphate. 2-Deoxyglucose (2DGlc), another glucose analogue that is non-metabolizable but is converted by hexokinase to 2DGlc 6-phosphate, at concentrations as low as 0.1 mM completely inhibited cell cycle progression of 2-cell embryos cultured in glucose-free (Glc(-)) medium with 10 microM phosphate. In contrast, in the absence of phosphate, 2DGlc at the same concentration allowed 55% of 2-cell embryos to develop to morula and blastocyst stages. Addition of an inhibitor of enolase in glycolysis, sodium fluoride (NaF), at 1 mM to the Glc(-) medium also enhanced the inhibitory effects of 10 microM phosphate, whereas 1 mM NaF in the absence of phosphate showed no inhibitory effects on the development of 2-cell embryos to morula and blastocyst stages. From these results, disturbance of glycolysis is a critical reason for the developmental inhibition caused by phosphate in early rat embryos in culture.

摘要

为了阐明磷酸盐诱导大鼠2细胞胚胎发育抑制的机制,我们研究了葡萄糖以及其他糖酵解和非糖酵解糖类、不可代谢的葡萄糖类似物和糖酵解抑制剂对磷酸盐抑制作用的相互影响。在没有葡萄糖的情况下,用10 - 500微摩尔磷酸盐处理的胚胎中有30 - 49%能够发育到桑葚胚和囊胚阶段。另一方面,在存在5毫摩尔葡萄糖的情况下,10微摩尔磷酸盐降低了2细胞胚胎发育到4细胞阶段的速率,并完全抑制了4细胞阶段之后的发育。相比之下,葡萄糖在无磷酸盐培养基中对发育没有影响。与葡萄糖类似,其他糖酵解糖类果糖(5毫摩尔)和甘露糖(5毫摩尔)增强了10微摩尔磷酸盐的抑制作用,但在没有磷酸盐的情况下没有影响。相反,非糖酵解糖类和不可代谢的葡萄糖类似物N - 乙酰葡糖胺和3 - O - 甲基葡萄糖(3 - O - MGlc)分别没有增强磷酸盐的作用。2 - 脱氧葡萄糖(2DGlc)是另一种不可代谢但可被己糖激酶转化为2 - 脱氧葡萄糖6 - 磷酸的葡萄糖类似物,在低至0.1毫摩尔的浓度下,它完全抑制了在含有10微摩尔磷酸盐的无葡萄糖(Glc(-))培养基中培养的2细胞胚胎的细胞周期进程。相比之下,在没有磷酸盐的情况下,相同浓度的2DGlc使55%的2细胞胚胎发育到桑葚胚和囊胚阶段。向Glc(-)培养基中添加1毫摩尔糖酵解中的烯醇化酶抑制剂氟化钠(NaF)也增强了10微摩尔磷酸盐的抑制作用,而在没有磷酸盐的情况下,1毫摩尔NaF对2细胞胚胎发育到桑葚胚和囊胚阶段没有抑制作用。从这些结果来看,糖酵解紊乱是培养的早期大鼠胚胎中磷酸盐导致发育抑制的关键原因。

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