AMPLIFIKASI PCR DOMAIN D1/D2 28S rDNA MENGGUNAKAN PRIMER ITS1 DAN ITS4 SAMPEL DNA DARI Candida tropicalis YANG DIISOLASI DENGAN METODE PENDINGINAN

H. Hermansyah, Novian Sutami, M. Miksusanti
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引用次数: 3

Abstract

The purpose of this research was to isolated DNA from the yeast C. tropicalis with freeze thawing method -200 C conducted on 3 colonies of C. tropicalis.  Each colony   threated variations of cooling, 3x15 minutes, 3x25 minutes and 3x35 minutes, to break the cell walls.  Subsequently all the samples amplified with 3 variations of PCR cycles, 15 cycles, 25 cycles and 35 cycles, after all of the samples isolated by freeze thawing method -200 C. Its was known that sample A15 has the smallest concentration of DNA yeast C. tropicalis, ie 50 µg/mL, while sample C35 had the largest concentration of DNA yeast C. tropicalis, ie 225 µg/mL. The result of the research indicated that the best condition can be reached in 3x35 minutes. On 35th cycle has clearer C. tropicalis DNA bands than the 25th and 15th PCR cycle. C. tropicalis DNA bands at 35th cycles there were 7 DNA bands were detected and bright bands on a long 35 minutes cooling. In the 25th and the 15th cycle, there was no DNA bands were detected in all samples. Based on the results obtained, the amplification process must be carried out at least 35 times cycles so that the C. tropicalis DNA bands can be detected.
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通过冷却方法对PCR域D1/D2 28S rDNA进行了抽样
本研究采用-200℃冻融法对3个热带酵母菌落进行DNA分离。每个菌落都有不同的冷却时间,分别是3x15分钟、3x25分钟和3x35分钟,以破坏细胞壁。所有样品经-200℃冻融法分离后,分别扩增15、25、35个PCR循环3个周期,得到样品A15的DNA酵母C. tropicalis浓度最小,为50µg/mL,样品C35的DNA酵母C. tropicalis浓度最大,为225µg/mL。研究结果表明,在3x35分钟内可达到最佳状态。与第25和第15个PCR周期相比,第35个PCR周期的热带镰刀菌DNA条带更清晰。经35次循环后,可检测到7条DNA条带,冷却35分钟后可检测到较亮的条带。在第25和第15个周期,所有样品均未检测到DNA条带。根据所获得的结果,扩增过程必须进行至少35次循环才能检测到热带镰刀菌的DNA条带。
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