This protocol describes thepolymerase chain reaction (PCR) setup and amplificationof bacterial16S rRNA genesusing27F and 1492R primers. The method utilizesPromega GoTaq® Green Master Mix (2x)and follows a standardthermal cycling programoptimized for bacterial DNA. Propersterile techniques, contamination prevention, and accurate pipettingare crucial to obtaining high-quality amplification results. The protocol includesnegative controlsto ensure reaction validity.
Ali et al. (Wed,) studied this question.
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