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脱氧胞苷可逆转胸苷对幼雏胚盘形态发生的抑制作用。

Deoxycytidine reverses inhibition of morphogenesis by thymidine in young chick blastoderm.

作者信息

Zagris N

出版信息

Teratog Carcinog Mutagen. 1986;6(3):203-8. doi: 10.1002/tcm.1770060305.

Abstract

Exogenous thymidine affects morphogenesis of the early chick blastoderm possibly by depleting the deoxycytidine triphosphate pool. The aim of this study is to determine whether the inhibitory action of thymidine on early chick blastoderm morphogenesis is alleviated by the removal of thymidine and/or treatment with deoxycytidine. Chick blastoderms at the full hypoblast stage develop abnormally in egg albumen containing 1.23 X 10(-3) M thymidine. Development is normal when deoxycytidine is included simultaneously in the culture medium with thymidine at equimolar concentrations. Blastoderms were cultured in egg albumen containing 15 microCi/ml thymidine [methyl-3H] or 10 microCi/ml deoxycytidine [5-3H], and 1.2 X 10(-3) M 2'-deoxycytidine or 1.23 X 10(-3) M thymidine, respectively. The culture was interrupted at timed intervals, and the amount of radioactivity associated with DNA was determined. Exogenous deoxycytidine in the culture medium caused a noticeable increase in the incorporation of 3H-thymidine, while exogenous thymidine markedly inhibited the uptake and incorporation of 3H-deoxycytidine into DNA of blastoderms. Thymidine does not inhibit the expansion of blastoderm, the migration of cells for formation of the primitive streak (PS), and the induction of axial tissues, but it interferes with the organization of these tissues to form the embryonic axis. Blastoderms show slight signs of recovery when thymidine is removed. Deoxycytidine counteracts the action of thymidine and seems to be a rate-limiting factor in normal differentiation of the early chick blastoderm.

摘要

外源性胸苷可能通过耗尽三磷酸脱氧胞苷库来影响早期鸡胚盘的形态发生。本研究的目的是确定去除胸苷和/或用脱氧胞苷处理是否能减轻胸苷对早期鸡胚盘形态发生的抑制作用。处于完全下胚层阶段的鸡胚盘在含有1.23×10⁻³ M胸苷的蛋清中发育异常。当在培养基中同时加入等摩尔浓度的胸苷和脱氧胞苷时,发育是正常的。胚盘分别在含有15 μCi/ml胸苷[甲基-³H]或10 μCi/ml脱氧胞苷[5-³H]以及1.2×10⁻³ M 2'-脱氧胞苷或1.23×10⁻³ M胸苷的蛋清中培养。在定时间隔中断培养,并测定与DNA相关的放射性量。培养基中的外源性脱氧胞苷导致³H-胸苷掺入量显著增加,而外源性胸苷则明显抑制³H-脱氧胞苷摄取并掺入胚盘DNA。胸苷并不抑制胚盘的扩展、细胞迁移形成原条(PS)以及轴向组织的诱导,但它会干扰这些组织形成胚胎轴的组织过程。当去除胸苷时,胚盘显示出轻微的恢复迹象。脱氧胞苷可抵消胸苷的作用,似乎是早期鸡胚盘正常分化中的一个限速因素。

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