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被猪鼻支原体污染的突变型HEp-2细胞系中的腺苷磷酸化酶活性

Adenosine phosphorylase activity in a mutant HEp-2 cell line contaminated with Mycoplasm hyorhinis.

作者信息

Thomas M A, Shipman C, Sandberg J N, Drach J C

出版信息

In Vitro. 1977 Aug;13(8):502-9. doi: 10.1007/BF02615143.

Abstract

Metabolic studies in HEp-2/MP,MIR cells (an adenosine kinase, hypoxanthine phosphoribosyltransferase negative mutant) indicated the presence of adenosine phosphorylase activity. This activity, unknown in established mammalian cell lines, resulted in the glycosidic cleavage of both adenosine and the antiviral drug arabinosyladenine. The activity was observed readily in the presence or absence of the adenosine deaminase inhibitor conformycin. Isopycnic separation of [3H] thymidine-labeled DNA species in CsCl density gradients resulted in the appearance of two distinct peaks. The heavier peak coincided with [14C]thymidine-labeled marker DNA of human origin, whereas the lighter peak was within the range associated with mycoplasmal DNA. Testing by commercial laboratories confirmed the presence of mycoplasma in HEp-2/MP,MIR cells. The contaminant was identified as Mycoplasma hyorhinis, a porcine mycoplasma. Following gamma-irradiation (3000 rads) to block cellular mitosis, the mucoplasma-contaminated HEp-2/MP,MIR cells were cocultivated with mycoplasma-free wild-type HEp-2 cells which did not exhibit adenosine phosphorylase activity. Following serial cocultivation in a medium designed to favor the survival of the wild-type cells, adenosine phosphorylase activity was found in the previously uninfected cells. Studies of this nature emphasize the need for investigators to carefully monitor their cell lines for mycoplasma.

摘要

在HEp-2/MP、MIR细胞(一种腺苷激酶、次黄嘌呤磷酸核糖转移酶阴性突变体)中的代谢研究表明存在腺苷磷酸化酶活性。这种活性在已建立的哺乳动物细胞系中并不为人所知,它导致腺苷和抗病毒药物阿糖腺苷的糖苷键断裂。无论是否存在腺苷脱氨酶抑制剂适形霉素,都能很容易地观察到这种活性。在CsCl密度梯度中对[3H]胸腺嘧啶标记的DNA物种进行等密度分离,结果出现了两个明显的峰。较重的峰与源自人类的[14C]胸腺嘧啶标记的标记DNA重合,而较轻的峰在与支原体DNA相关的范围内。商业实验室的检测证实HEp-2/MP、MIR细胞中存在支原体。污染物被鉴定为猪鼻支原体,一种猪支原体。在进行γ射线照射(3000拉德)以阻断细胞有丝分裂后,将受支原体污染的HEp-2/MP、MIR细胞与不具有腺苷磷酸化酶活性的无支原体野生型HEp-2细胞共培养。在一种有利于野生型细胞存活的培养基中进行连续共培养后,在先前未感染的细胞中发现了腺苷磷酸化酶活性。这种性质的研究强调了研究人员需要仔细监测他们的细胞系是否存在支原体。

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