Validation and characterization of murine gammaherpesvirus 68 antisense transcripts by northern blot analysis and quantitative reverse transcription-PCR

Pub Date : 2023-01-01 DOI:10.2298/abs230407016k
M. Kara
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Abstract

The transcription of mammalian genomes exhibits an intriguing complexity and numerous novel RNA molecules have been identified. Viruses with large DNA genomes, especially herpesviruses, generate many different RNA species, including long non-coding RNAs (lncRNAs). Dense viral genomes can generate multigenic transcripts in addition to commonly observed antisense transcripts. It is essential to study the biological roles of these transcripts aside from the protein-coding counterparts. Multiple antisense transcripts from the open reading frame (ORF) 63-64 locus in murine gammaherpesvirus 68 (MHV68) were detected by northern blotting. Expression analysis by quantitative reverse transcription PCR (qRT-PCR) did not detect different isoforms. Several alternative splicing isoforms exist during lytic replication; however, they are not detected during latency. To identify the roles of these new transcripts, qRT-PCR may not be enough and should be supported by an alternative method such as northern blotting. A more detailed transcriptional map of the locus of interest is useful to design experimental strategies and perform functional studies, especially when working with gene-dense viral genomes.
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小鼠γ疱疹病毒68反义转录物的northern blot和定量逆转录pcr验证和鉴定
哺乳动物基因组的转录表现出一种有趣的复杂性,许多新的RNA分子已经被确定。具有大DNA基因组的病毒,特别是疱疹病毒,产生许多不同种类的RNA,包括长链非编码RNA (lncRNAs)。除了常见的反义转录物外,密集的病毒基因组还可以产生多基因转录物。除了蛋白质编码对应物外,研究这些转录本的生物学作用是至关重要的。用northern印迹法检测了鼠γ疱疹病毒68 (MHV68)开放阅读框(ORF) 63-64位点的多个反义转录本。定量反转录PCR (qRT-PCR)表达分析未检测到不同亚型。在裂解复制过程中存在几种不同的剪接异构体;但是,它们在延迟期间不会被检测到。为了确定这些新转录本的作用,qRT-PCR可能还不够,应该采用其他方法,如northern blotting。更详细的兴趣位点转录图谱有助于设计实验策略和进行功能研究,特别是在处理基因密集的病毒基因组时。
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