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低pH值对各种培养的哺乳动物细胞的致断裂性

Clastogenicity of low pH to various cultured mammalian cells.

作者信息

Morita T, Nagaki T, Fukuda I, Okumura K

机构信息

Tsukuba Research Laboratories, Nippon Glaxo Ltd., Ibaraki, Japan.

出版信息

Mutat Res. 1992 Aug;268(2):297-305. doi: 10.1016/0027-5107(92)90235-t.

Abstract

It has been reported that low pH itself can be clastogenic to Chinese hamster ovary cells or mouse lymphoma L5178Y cells. On the other hand, there was no indication that low pH is clastogenic to rat or human lymphocytes. Therefore, in order to evaluate the generality of clastogenicity of low pH conditions, chromosomal aberration tests were carried out on Chinese hamster cell line cells (CHO-K1, CHL, Don and V79 379A) and human cells (HeLa and peripheral lymphocytes used as whole-blood cultures). The cytotoxicity of low pH to each cell line was also evaluated by counting surviving cells. The treatment medium used was Eagle's MEM containing 15 mM MES or Bis-Tris as an organic buffer to maintain the acidity of the medium for the 6-h or 24-h treatment period, and pH adjustment was done with NaOH or HCl. Chromosomal aberrations were induced at pH 6.5 or below in CHO or CHL cells, and the maximum frequency was 24.7% at pH 6.0 or 34% at pH 6.3, respectively. About 5-10% of Don or HeLa cells had aberrations over the range of pH 6.6-6.0 or pH 6.6-6.3, respectively. In V79 379A cells or human lymphocytes, however, aberrant cells amounted to about 8% at near pH 6.0, where cell survival was low (less than 20%). About 90% of aberrations induced in each cell line examined were chromatid-type gaps and breaks. When CHO or CHL cells were treated with acidic medium for 6 h plus 18 h recovery in fresh medium, about 20% of cells had aberrations including chromatid exchanges at pH 5.5 or pH 5.7, respectively. These results indicate that clastogenicity of low pH is a general finding, although the extent of it varies with cell type, and that the clastogenicity is associated with varying extents of cytotoxicity. The mechanisms of clastogenesis at low pH are not known, but might involve inhibition of DNA or protein synthesis or DNA-repair enzymes.

摘要

据报道,低pH值本身可对中国仓鼠卵巢细胞或小鼠淋巴瘤L5178Y细胞具有致断裂作用。另一方面,没有迹象表明低pH值对大鼠或人淋巴细胞有致断裂作用。因此,为了评估低pH条件下致断裂作用的普遍性,对中国仓鼠细胞系细胞(CHO-K1、CHL、Don和V79 379A)和人细胞(HeLa细胞以及用作全血培养的外周血淋巴细胞)进行了染色体畸变试验。还通过计数存活细胞来评估低pH值对每种细胞系的细胞毒性。所用的处理培养基是含有15 mM MES或Bis-Tris作为有机缓冲剂的Eagle's MEM培养基,以便在6小时或24小时的处理期间维持培养基的酸度,并用NaOH或HCl进行pH调节。在CHO或CHL细胞中,pH值为6.5或更低时可诱导染色体畸变,在pH值为6.0时最大频率为24.7%,在pH值为6.3时为34%。在pH值6.6 - 6.0或pH值6.6 - 6.3范围内,分别约有5 - 10%的Don或HeLa细胞出现畸变。然而,在V79 379A细胞或人淋巴细胞中,在接近pH值6.0时畸变细胞约占8%,此时细胞存活率较低(低于20%)。在所检测的每种细胞系中,约90%的诱导畸变是染色单体型的间隙和断裂。当CHO或CHL细胞用酸性培养基处理6小时后,再在新鲜培养基中恢复18小时,在pH值5.5或pH值5.7时,分别约有20%的细胞出现包括染色单体交换在内的畸变。这些结果表明,低pH值的致断裂作用是一个普遍现象,尽管其程度因细胞类型而异,并且致断裂作用与不同程度的细胞毒性相关。低pH值下致断裂的机制尚不清楚,但可能涉及对DNA或蛋白质合成或DNA修复酶的抑制。

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