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吖啶橙染色法在聚丙烯酰胺凝胶中检测轮状病毒RNA的应用。

Use of acridine orange staining for the detection of rotavirus RNA in polyacrylamide gels.

作者信息

Lauretti Flávio, Lucas de Melo Fernando, Benati Fabrício José, de Mello Volotão Eduardo, Santos Norma, Linhares Rosa Elisa Carvalho, Nozawa Carlos

机构信息

Departamento de Microbiologia, Centro de Ciências Biológicas, Universidade Estadual de Londrina, CEP 86051-900, Londrina, Paraná, Brazil.

出版信息

J Virol Methods. 2003 Dec;114(1):29-35. doi: 10.1016/j.jviromet.2003.08.005.

Abstract

Acridine orange is a metachromatic intercalator used extensively in histochemistry to differentiate double- from single-stranded (ds, ss) nucleic acid by the emission of green and red fluorescence, respectively, under ultraviolet light. In the present study we standardised a protocol in order to use acridine orange to detect rotavirus ds RNA in polyacrylamide gels and compared it to silver and ethidium bromide staining. We demonstrated that the simplest and best condition was attained when gels containing rotavirus ds RNA bands, stained in green, were treated with 4.3 microM acridine orange after electrophoresis and destained with distilled water pH 6 at 37 degrees C. Under this protocol, rotavirus RNA concentration was calculated and the mean minimum amounts of nucleic acid detected by acridine orange, ethidium bromide, and silver staining were 26.0 +/- 4.29, 15.6 +/- 1.48 and 1.06 +/- 0.11 ng, respectively. The comparison of acridine orange sensitivity with ethidium bromide and silver staining, for 25 field strains of rotavirus and one cell-adapted strain (SA11), demonstrated concurrent results in 80% of the specimens. Red colour emission resulting from the interaction of acridine orange with ss nucleic acid was also shown by testing denatured 0.5 kb HindIII digest of lambda phage DNA. Furthermore, it was demonstrated that rotavirus ds RNA could be used for reverse transcription activity, followed by PCR amplification, after acridine orange staining. In conclusion, although acridine orange is less sensitive than ethidium bromide and silver staining, its practicality, low cost, metachromatic properties, and its non-interference on RT-PCR should be considered. It is suggested the use of acridine orange as an appropriate stain for various purposes in virology, as well as for the molecular biology of nucleic acid.

摘要

吖啶橙是一种异染性嵌入剂,在组织化学中广泛应用,通过在紫外光下分别发出绿色和红色荧光来区分双链和单链核酸。在本研究中,我们标准化了一种方案,以便使用吖啶橙检测聚丙烯酰胺凝胶中的轮状病毒双链RNA,并将其与银染和溴化乙锭染色进行比较。我们证明,当含有绿色染色的轮状病毒双链RNA条带的凝胶在电泳后用4.3微摩尔/升的吖啶橙处理,并在37℃下用pH 6的蒸馏水脱色时,可达到最简单和最佳的条件。按照该方案计算了轮状病毒RNA浓度,吖啶橙、溴化乙锭和银染检测到的核酸平均最小量分别为26.0±4.29、15.6±1.48和1.06±0.11纳克。对25株轮状病毒野毒株和1株细胞适应株(SA11)进行吖啶橙敏感性与溴化乙锭和银染的比较,结果显示80%的标本结果一致。通过检测变性的λ噬菌体DNA 0.5 kb HindIII酶切产物,也证明了吖啶橙与单链核酸相互作用产生的红色荧光。此外,还证明了轮状病毒双链RNA在吖啶橙染色后可用于逆转录活性,随后进行PCR扩增。总之,尽管吖啶橙的敏感性低于溴化乙锭和银染,但其实用性、低成本、异染特性以及对逆转录-聚合酶链反应无干扰等优点应予以考虑。建议将吖啶橙用作病毒学以及核酸分子生物学中各种用途的合适染色剂。

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