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B细胞淋巴瘤DNA中N-ras基因与unr基因之间的鼠白血病病毒前病毒插入仅影响N-ras的表达。

Murine leukemia virus proviral insertions between the N-ras and unr genes in B-cell lymphoma DNA affect the expression of N-ras only.

作者信息

Martín-Hernández J, Sørensen A B, Pedersen F S

机构信息

Department of Molecular and Structural Biology, University of Aarhus, DK-8000 Aarhus C, Denmark.

出版信息

J Virol. 2001 Dec;75(23):11907-12. doi: 10.1128/JVI.75.23.11907-11912.2001.

Abstract

Akv1-99, a variant of Akv murine leukemia virus, induces B-cell lymphomas with nearly 100% incidence and a mean latency period of 12 months after injection into newborn NMRI mice. PCR amplification and sequence analyses of DNA flanking integrated proviruses revealed proviral insertion into the N-ras/unr (upstream of N-ras) locus in 2 out of 13 B-cell lymphomas, both of which appeared clonal by Southern blotting analysis. These two tumors showed increased expression levels of N-ras by Northern blotting, as did a third tumor shown by reverse transcriptase PCR to have a nonclonal provirus integration located in the same area. However, no significant changes in expression were observed when using a specific probe for the unr gene. All proviruses were integrated in the same transcriptional orientation as unr and N-ras genes. By promoter insertion, the two Akv1-99 proviruses integrated between exon -1 and exon 1 of N-ras gave rise to two different spliced products, whereas the provirus integrated into unr used only an exon skipping pattern. The absence of mutations of the N-ras codons 12, 13, 18, and 61 suggests that activation of the proto-oncogene is exclusively due to overexpression by retroviral promoter insertion, and furthermore, Northern blot analyses indicate that the expression of unr is unaffected by N-ras overexpression even in the case where the unr gene itself is the target of proviral insertion. Thus, altogether our findings indicate that overexpression of N-ras plays a role in development of murine leukemia virus-induced B-cell lymphomas, leaving the expression of the tightly linked unr gene unaltered.

摘要

Akv1-99是Akv鼠白血病病毒的一种变体,将其注射到新生NMRI小鼠体内后,可诱发B细胞淋巴瘤,发病率近100%,平均潜伏期为12个月。对整合的原病毒侧翼DNA进行PCR扩增和序列分析,结果显示,在13个B细胞淋巴瘤中有2个的原病毒插入到了N-ras/unr(N-ras上游)基因座,通过Southern印迹分析,这两个淋巴瘤均呈现克隆性。通过Northern印迹分析发现,这两个肿瘤中N-ras的表达水平升高,通过逆转录酶PCR分析显示,第三个肿瘤的原病毒非克隆性整合位于同一区域,其N-ras表达水平也升高。然而,当使用针对unr基因的特异性探针时,未观察到表达有显著变化。所有原病毒均以与unr和N-ras基因相同的转录方向整合。通过启动子插入,整合到N-ras外显子-1和外显子1之间的两个Akv1-99原病毒产生了两种不同的剪接产物,而整合到unr中的原病毒仅采用外显子跳跃模式。N-ras密码子12、13、18和61未发生突变,这表明原癌基因的激活完全是由于逆转录病毒启动子插入导致的过表达,此外,Northern印迹分析表明,即使在unr基因本身是原病毒插入靶点的情况下,unr的表达也不受N-ras过表达的影响。因此,我们的研究结果总体表明,N-ras的过表达在鼠白血病病毒诱导的B细胞淋巴瘤的发生中起作用,而紧密连锁的unr基因的表达未发生改变。

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