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The use of fluorescein diacetate to assess embryo viability in the mouse

机译:使用双乙酸荧光素评估小鼠胚胎的存活力

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Summary. Preimplantation mouse embryos that were exposed to fluorescein diacetate (FDA) accumulated intracellular fluorescein and fluoresced brightly under ultraviolet (u.v.) light. The rate at which intracellular fluorescein was lost from the cells was measured at 37, 28 and 4°C and the rate decreased as the storage temperature decreased. The rate at which intracellular fluorescein accumulated increased as FDA concentration increased until a maximum rate was attained. The ability to accumulate intracellular fluorescein could be removed by heating embryos at 56°C for 30 min or by damaging the cell membrane. Cells grown under inadequate culture conditions lost the ability to accumulate intracellular fluorescein. Exposure of 2-cell mouse embryos to FDA and u.v. light did not alter the rate of blastocyst formation in vitro, and exposure of blastocysts to FDA and u.v. light did not alter the rate of implantation or post-implantation development in vivo.
机译:概要。暴露于二乙酸荧光素(FDA)的植入前小鼠胚胎会积聚细胞内荧光素,并在紫外(u.v.)光下发出明亮的荧光。在37、28和4℃下测量细胞内荧光素从细胞中丢失的速率,并且该速率随着储存温度的降低而降低。细胞内荧光素积累的速率随FDA浓度的增加而增加,直至达到最大速率。可以通过将胚胎在56°C加热30分钟或破坏细胞膜来消除积累细胞内荧光素的能力。在不足的培养条件下生长的细胞失去了积累细胞内荧光素的能力。将2细胞小鼠胚胎暴露于FDA和u.v.光照不会改变体外胚泡的形成速度,并且胚泡暴露于FDA和u.v。光不会改变体内植入或植入后发育的速率。

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