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Hi,
About half our samples post library prep (poly(A) selection) + sequencing had around 50% rRNA content. The samples were re-prepped in the facility but the rRNA contents were similar a second time.
The facility now argue that the rRNA "contamination" is sample related and not due to failed library prep. Since the poly(A) selection enriches for all RNAs that have a poly(A) tail, mostly mRNAs, rRNA removal should have been effective? What can have gone wrong?
The tissue is skin and we used mirVana kit to extract RNA (perhaps not optimal - could the inclusion of small RNAs caused an issue in the library prep?). All our samples had RIN of 8 and above.
Thanks in advance!
About half our samples post library prep (poly(A) selection) + sequencing had around 50% rRNA content. The samples were re-prepped in the facility but the rRNA contents were similar a second time.
The facility now argue that the rRNA "contamination" is sample related and not due to failed library prep. Since the poly(A) selection enriches for all RNAs that have a poly(A) tail, mostly mRNAs, rRNA removal should have been effective? What can have gone wrong?
The tissue is skin and we used mirVana kit to extract RNA (perhaps not optimal - could the inclusion of small RNAs caused an issue in the library prep?). All our samples had RIN of 8 and above.
Thanks in advance!
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