Optimization of PCR Protocols for ITS rDNA Amplification of Yeasts Isolated from Apis mellifera Honeycomb

Ayudya Fitri Arifa, N. F. Firdhausi, Irul Hidayati, Y. Rachmawati, M. Hadi
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Abstract

Yeast is a microorganism that can be found in honeycomb. Yeast identification is a process to find and identify new species. One of which is molecular identification of yeast with rDNA sequences in the ITS region. Before carrying out molecular identification, it is necessary to optimize yeast DNA amplification methods to obtain good DNA sequences that ease the yeast identification process. The purpose of this study was to discover the optimum PCR (Polymerase Chain Reaction)protocols for the identification of yeasts isolated from Apis mellifera honeycomb based on the ITS rDNA. This study used 3 PCR (Polymerase Chain Reaction) protocols, i.e., from Kanti et al. (2018), Ediningsari (2008), and Maulana (2011). This results study shows that the optimum PCR protocol was from Maulana (2011), which produced clear and whole DNA fragment luminescences.
蜜蜂蜂巢酵母ITS rDNA扩增方法的优化
酵母是一种可以在蜂窝中找到的微生物。酵母鉴定是一个发现和鉴定新物种的过程。其中之一是酵母ITS区rDNA序列的分子鉴定。在进行分子鉴定之前,有必要优化酵母DNA扩增方法,以获得良好的DNA序列,从而简化酵母鉴定过程。本研究旨在探索基于ITS rDNA的蜜蜂蜂窝酵母最佳PCR (Polymerase Chain Reaction,聚合酶链反应)鉴定方案。本研究使用了3种PCR(聚合酶链反应)方案,即来自Kanti等人(2018)、Ediningsari(2008)和Maulana(2011)。本研究结果表明,最佳PCR方案来自Maulana(2011),该方案产生清晰且完整的DNA片段发光。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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