Raw sequence reads from healthy human blood samples

The protocol used in this study intended to enrich viral fraction in order to characterize human virome from healthy blood donors using different experimental combinations. In this study, we compared direct extraction methods with strategies involving filtration and centrifugation steps. We used nucleases to remove free nucleic acids and independent viral DNA and RNA extraction were performed, followed by a random amplification and library preparation.Sample description:M1: Direct extraction + filtered with 0.45 micrometers, DNA libraryM2: Direct extraction + filtered with 1 micrometers, DNA libraryM3: High centrifugation + filtered with 0.45 micrometers, DNA libraryM4: High centrifugation + filtered with 1 micrometers (P1), DNA library. This sample is also P1.M5: Direct extraction + filtered with 0.45 micrometers, RNA libraryM6: Direct extraction + filtered with 0.45 micrometers, RNA libraryM7: High centrifugation + filtered with 0.45 micrometers, RNA libraryM8: High centrifugation + filtered with 1 micrometers, RNA libraryP2-P12: High centrifugation + filtered with 0.45 and 1 micrometers, DNA and RNA library