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Dears:
i am using the KAPA Stranded RNA-Seq
Library Preparation Kit to prepare my Libraries from RNA starting material. i had a very good success rate using this kit , but yesterday after the PCR amplification step and clean up step with the beads the qubit concentration of my libraries was in the range of 1-19 ng/ul. but in the bioanalyzer i had no peaks for my libraries . any suggestions? and this is the first time it happened with me ???
i am using the KAPA Stranded RNA-Seq
Library Preparation Kit to prepare my Libraries from RNA starting material. i had a very good success rate using this kit , but yesterday after the PCR amplification step and clean up step with the beads the qubit concentration of my libraries was in the range of 1-19 ng/ul. but in the bioanalyzer i had no peaks for my libraries . any suggestions? and this is the first time it happened with me ???
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