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海星卵母细胞减数分裂成熟过程中及激活后核糖体蛋白的磷酸化:其与细胞内pH变化的关系

Phosphorylation of ribosomal proteins during meiotic maturation and following activation in starfish oocytes: its relationship with changes of intracellular pH.

作者信息

Peaucellier G, Picard A, Robert J J, Capony J P, Labbe J C, Doree M

机构信息

Station Biologique, Roscoff, France.

出版信息

Exp Cell Res. 1988 Jan;174(1):71-88. doi: 10.1016/0014-4827(88)90143-7.

Abstract

An increased phosphorylation of ribosomal protein S6 has been shown to be correlated with an increase of intracellular pH (pHi) and with stimulation of protein synthesis in many systems. In this research changes in ribosome phosphorylation following hormone-induced meiotic maturation and fertilization or activation by ionophore A23187 were investigated in starfish oocytes. The hormone was found to stimulate, even in the absence of external Na+, the phosphorylation on serine residues of an Mr 31,000 protein identified as S6, as well as that of an acidic Mr 47,000 protein, presumably S1, on threonine residues. Phosphorylation of ribosomes was an early consequence of hormonal stimulation and did not decrease after completion of meiotic maturation. Fertilization or activation by ionophore of prophase-arrested oocytes also stimulated ribosome phosphorylation. Only S6 was labeled in this case, but to a lesser extent than upon hormone-induced meiotic maturation. Changes in pHi were monitored with ion-specific microelectrodes throughout meiotic maturation and following either fertilization or activation. The pHi did not change before germinal vesicle breakdown (GVBD) following hormone addition, but it increased before first polar body emission. It also increased following fertilization or activation by ionophore or the microinjection of Ca-EGTA. In all cases, alkalinization did not depend on activation of an amiloride-sensitive Na+/H+ exchanger. Microinjection of an alkaline Hepes buffer or external application of ammonia, both of which increased pHi, prevented unfertilized oocytes from arresting after formation of the female pronucleus and induced chromosome cycling. Phosphorylation of S6 was still observed following fertilization or induction of maturation when pHi was decreased by external application of acetate, a treatment which suppressed the emission of polar bodies. Protein synthesis increased in prophase-arrested oocytes after fertilization or activation. It also increased after ammonia addition, although this treatment did not stimulate S6 phosphorylation.

摘要

核糖体蛋白S6磷酸化增加已被证明与许多系统中细胞内pH值(pHi)升高以及蛋白质合成的刺激相关。在本研究中,研究了海星卵母细胞中激素诱导的减数分裂成熟、受精或离子载体A23187激活后核糖体磷酸化的变化。发现该激素即使在没有外部Na+的情况下,也能刺激被鉴定为S6的31,000 Mr蛋白丝氨酸残基上的磷酸化,以及酸性47,000 Mr蛋白(可能是S1)苏氨酸残基上的磷酸化。核糖体磷酸化是激素刺激的早期结果,减数分裂成熟完成后并未降低。前期阻滞的卵母细胞受精或离子载体激活也会刺激核糖体磷酸化。在这种情况下,只有S6被标记,但程度低于激素诱导的减数分裂成熟。在整个减数分裂成熟过程中以及受精或激活后,用离子特异性微电极监测pHi的变化。添加激素后,在生发泡破裂(GVBD)之前pHi没有变化,但在第一极体排出之前升高。受精或离子载体激活或微量注射Ca-EGTA后也会升高。在所有情况下,碱化不依赖于氨氯地平敏感的Na+/H+交换器的激活。微量注射碱性Hepes缓冲液或外部施加氨,两者都会升高pHi,可防止未受精卵母细胞在雌原核形成后停滞并诱导染色体循环。当通过外部施加醋酸盐降低pHi时,受精或诱导成熟后仍可观察到S6磷酸化,这种处理抑制了极体的排出。受精或激活后,前期阻滞的卵母细胞中蛋白质合成增加。添加氨后也增加,尽管这种处理不会刺激S6磷酸化。

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