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在非病毒病因的BALB/c肿瘤细胞系中检测小鼠乳腺肿瘤病毒RNA。

Detection of mouse mammary tumor virus RNA in BALB/c tumor cell lines of nonviral etiologies.

作者信息

Dudley J P, Butel J S, Socher S H, Rosen J M

出版信息

J Virol. 1978 Dec;28(3):743-52. doi: 10.1128/JVI.28.3.743-752.1978.

Abstract

A complementary DNA (cDNA) probe to mouse mammary tumor virus (MMTV) RNA was synthesized using calf thymus DNA oligonucleotides as a random primer. This probe was then used to study the expression of MMTV RNA in cell lines from BALB/c tumors induced in vivo either spontaneously or in response to viral, chemical, or hormonal stimuli. The cDNA had a length of approximately 400 to 500 nucleotides and specifically hybridized to MMTV RNA and BALB/c lactating mammary gland RNA, but not to Moloney leukemia virus RNA. Calf thymus DNA-primed cDNA could protect 50% of iodinated MMTV RNA from S1 nuclease digestion at cDNA-RNA ratios of 1:1 and 90% of labeled viral RNA at ratios of 10:1. Thermal denaturation of MMTV RNA-cDNA hybrids yielded a T(m) of 88.5 degrees C, indicative of a well-base-paired duplex. Screening of mouse mammary tumor cells for MMTV sequences revealed that three out of five lines of BALB/c origin had undetectable levels of viral RNA (<three molecules per cell) by RNA excess hybridization. Two of the three "virus-negative" cell lines were derived from tumors induced by the chemical carcinogen 7,12-dimethylbenz(alpha)anthracene, whereas the third tumor occurred spontaneously. Two lines from tumors induced by either viral (mammary tumor virus) or hormonal (17-beta-estradiol) stimulus contained between three and nine molecules of MMTV RNA per cell by both RNA excess and cDNA excess hybridization. Clonal derivatives of these tumor lines had levels of viral RNA comparable to those of their parental lines. Therefore, it appears that the presence of detectable MMTV RNA sequences is not a necessary requirement for the maintenance of all murine mammary gland neoplasias.

摘要

使用小牛胸腺DNA寡核苷酸作为随机引物合成了小鼠乳腺肿瘤病毒(MMTV)RNA的互补DNA(cDNA)探针。然后使用该探针研究MMTV RNA在BALB/c小鼠体内自发诱导或对病毒、化学或激素刺激产生反应而诱导产生的肿瘤细胞系中的表达。该cDNA长度约为400至500个核苷酸,可特异性杂交至MMTV RNA和BALB/c泌乳乳腺RNA,但不与莫洛尼白血病病毒RNA杂交。以小牛胸腺DNA为引物的cDNA在cDNA与RNA比例为1:1时可保护50%的碘化MMTV RNA不被S1核酸酶消化,在比例为10:1时可保护90%的标记病毒RNA。MMTV RNA-cDNA杂交体的热变性产生的熔解温度(T(m))为88.5℃,表明双链碱基配对良好。对小鼠乳腺肿瘤细胞进行MMTV序列筛选发现,在五个源自BALB/c的细胞系中,有三个通过RNA过量杂交检测不到病毒RNA水平(每个细胞<三个分子)。三个“病毒阴性”细胞系中的两个源自化学致癌物7,12-二甲基苯并(α)蒽诱导的肿瘤,而第三个肿瘤是自发产生的。通过RNA过量杂交和cDNA过量杂交,由病毒(乳腺肿瘤病毒)或激素(17-β-雌二醇)刺激诱导产生的肿瘤的两个细胞系每个细胞含有三至九个MMTV RNA分子。这些肿瘤细胞系的克隆衍生物的病毒RNA水平与其亲本细胞系相当。因此,似乎可检测到的MMTV RNA序列的存在并非维持所有小鼠乳腺肿瘤所必需。

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