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在5-溴脱氧尿苷一轮DNA合成后对成肌细胞融合的抑制作用。

Inhibition of myoblast fusion after one round of DNA synthesis in 5-bromodeoxyuridine.

作者信息

Bischoff R, Holtzer H

出版信息

J Cell Biol. 1970 Jan;44(1):134-50. doi: 10.1083/jcb.44.1.134.

Abstract

The thymidine analogue 5-bromodeoxyuridine (BUdR) has a differential effect on the synthesis of tissue-specific products and molecules required for growth and division. Proliferating myogenic cells cultured in BUdR fail to fuse and fail to initiate the synthesis of contractile protein filaments. Conversely, BUdR has but a minor effect on cell viability and reproductive integrity. Low concentrations of BUdR result in an enhancement of cell number relative to the controls; higher concentrations are cytotoxic. Suppression of myogenesis is reversible after at least 10 cell generations of growth in the analogue. Cells that do not synthesize DNA, such as postmitotic myoblasts and myotubes, are not affected by BUdR. Incorporation of BUdR for one round of DNA synthesis was accomplished by first incubating myogenic cells, prior to fusion, in 5-fluorodeoxyuridine (FUdR) to block DNA synthesis and collect cells in the presynthetic phase. The cells were then allowed to synthesize either normal DNA or BU-DNA for one S period by circumventing the FUdR block with BUdR or BUdR plus thymidine (TdR). The cultures were continued in FUdR to prevent dilution of the incorporated analogue by further division. After 3 days, the cultures from the FUdR-BUdR series showed the typical BUdR effect; the cells were excessively flattened and few multinucleated myotubes formed. Cells in the control cultures were of normal morphology, and multinucleated myotubes were present. These results were confirmed in another experiment in which BUdR-(3)H was added to 2-day cultures in which myotubes were forming. Fusion of thymidine-(3)H-labeled cells begins at 8 hr after the preceding S phase. In contrast, cells which incorporate BUdR-(3)H for one S period do not fuse with normal myotubes.

摘要

胸苷类似物5-溴脱氧尿苷(BUdR)对组织特异性产物以及生长和分裂所需分子的合成具有不同的影响。在含有BUdR的培养基中培养的增殖性成肌细胞无法融合,也无法启动收缩蛋白丝的合成。相反,BUdR对细胞活力和生殖完整性的影响较小。低浓度的BUdR相对于对照组会导致细胞数量增加;高浓度则具有细胞毒性。在类似物中生长至少10个细胞代后,肌生成的抑制作用是可逆的。不合成DNA的细胞,如有丝分裂后的成肌细胞和肌管,不受BUdR影响。通过在融合前先将成肌细胞在5-氟脱氧尿苷(FUdR)中孵育以阻断DNA合成,并收集处于合成前期的细胞,从而实现一轮DNA合成中BUdR的掺入。然后通过用BUdR或BUdR加胸苷(TdR)绕过FUdR阻断,使细胞合成正常DNA或BU-DNA一个S期。培养物继续在FUdR中培养,以防止掺入的类似物因进一步分裂而被稀释。3天后,来自FUdR-BUdR系列的培养物表现出典型的BUdR效应;细胞过度扁平,几乎没有形成多核肌管。对照培养物中的细胞形态正常,存在多核肌管。在另一项实验中证实了这些结果,在该实验中,将BUdR-(3)H添加到正在形成肌管的2天龄培养物中。胸腺嘧啶核苷-(3)H标记的细胞在前一个S期后8小时开始融合。相比之下,掺入BUdR-(3)H一个S期的细胞不会与正常肌管融合。

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