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罗司维汀处理可改善供体细胞周期在G0/G1期的同步性以及手工克隆水牛胚胎的体外发育。

Roscovitine treatment improves synchronization of donor cell cycle in G0/G1 stage and in vitro development of handmade cloned buffalo (Bubalus bubalis) embryos.

作者信息

Selokar Naresh L, Saini Monika, Muzaffer Mushariffa, Krishnakanth G, Saha Ambika P, Chauhan Manmohan S, Manik Radheysham, Palta Prabhat, Madan Pavneesh, Singla Suresh K

机构信息

Animal Biotechnology Centre, National Dairy Research Institute, Karnal, India.

出版信息

Cell Reprogram. 2012 Apr;14(2):146-54. doi: 10.1089/cell.2011.0076. Epub 2012 Feb 28.

Abstract

This study investigated the effects of serum-starvation, total confluence, and roscovitine treatment on cell-cycle synchronization of buffalo ear skin fibroblasts to the G0/G1 stage and on the developmental competence of cloned embryos. Serum starvation of total confluence cultures for 24 h had a higher (p<0.05) proportion of cells at G0/G1 stage (94.4%) compared with serum starved cyclic and nonstarved confluent cultures (76.8 and 86.0%, respectively), whereas differences between cyclic cells with or without serum starvation were not significant. The proportion of cells at G0/G1 was higher (p<0.05) with 20 and 30 μM roscovitine treatment than that with 10 μM (94.4, 96.4, and 86.6%, respectively), which was similar to that for total confluence (86.0%). MTT assay showed that cell viability decreased as dose of roscovitine increased. The blastocyst rate was significantly higher (p<0.05) when nuclear transfer embryos were reconstructed using donors cells from total confluence, confluence serum starved, and roscovitine-treated (20 and 30 μM) groups (48.8, 48.9, 57.9, and 62.9%, respectively) compared to nontreated cyclic cells (20.2%). However, the cleavage rate and total cell number of cloned embryos were similar for all the groups. The number of ICM cells was improved by 30 μM roscovitine treatment (45.25 ± 2.34). The cryosurvival rate of blastocysts derived from cells synchronized with 20 or 30 μM roscovitine was higher compared to that for total confluence group (33.6, 37.8 vs. 23.8%). In conclusion, treatment with 30 μM roscovitine is optimal for harvesting G0/G1 stage cells for producing high quality cloned buffalo embryos, and that it is better than serum-starvation or total confluence for cell synchronization.

摘要

本研究调查了血清饥饿、完全汇合及罗哌卡因处理对水牛耳皮肤成纤维细胞细胞周期同步至G0/G1期以及对克隆胚胎发育能力的影响。与血清饥饿的周期性培养细胞和未饥饿的汇合培养细胞(分别为76.8%和86.0%)相比,完全汇合培养物血清饥饿24小时后处于G0/G1期的细胞比例更高(p<0.05)(94.4%),而血清饥饿的周期性细胞与未饥饿的周期性细胞之间的差异不显著。20 μM和30 μM罗哌卡因处理组处于G0/G1期的细胞比例高于10 μM处理组(分别为94.4%、96.4%和86.6%),差异显著(p<0.05),这与完全汇合组(86.0%)相似。MTT分析表明,细胞活力随罗哌卡因剂量增加而降低。当使用来自完全汇合、汇合血清饥饿及罗哌卡因处理(20 μM和30 μM)组的供体细胞重建核移植胚胎时,囊胚率显著更高(p<0.05)(分别为48.8%、48.9%、57.9%和62.9%),相比之下,未处理的周期性细胞组为20.2%。然而,所有组克隆胚胎的裂解率和总细胞数相似。30 μM罗哌卡因处理可提高内细胞团细胞数量(45.25±2.34)。与完全汇合组相比,用20 μM或30 μM罗哌卡因同步化的细胞来源的囊胚冷冻存活率更高(分别为33.6%、37.8%对23.8%)。总之,30 μM罗哌卡因处理最适合收获G0/G1期细胞以生产高质量的克隆水牛胚胎,并且在细胞同步化方面优于血清饥饿或完全汇合。

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