SRX22328660
GSM7876399_r1
GSM7876399: N2_Untreated [Control]; Caenorhabditis elegans; RNA-Seq
SRP469661
PRJNA1034565
SRS19378686
GSM7876399
GSM7876399
RNA-Seq
TRANSCRIPTOMIC
cDNA
Total RNA was extracted from whole nematodes using TRIzol kit (Invitrogen). Oligo(dT)-attached magnetic beads were used to purified mRNA. Purified mRNA was fragmented into small pieces with fragment buffer at appropriate temperature. Then first-strand cDNA was generated using random hexamer-primed reverse transcription, followed by a second-strand cDNA synthesis. Afterwards, A-Tailing Mix and RNA Index Adapters were added by incubating to end repair. The cDNA fragments obtained from previous step were amplified by PCR, and products were purified by Ampure XP Beads, then dissolved in EB solution. The product was validated on the Agilent Technologies 2100 bioanalyzer for quality control. The double stranded PCR products from previous step were heated denatured and circularized by the splint oligo sequence to get the final library. The single strand circle DNA was formatted as the final library. The final library was amplified with phi29 to make DNA nanoball which had more than 300 copies of one molecular, DNBs were loaded into the patterned nanoarray and pair end 100 bases reads were generated on BGIseq500 platform (BGI-Shenzhen, China).
BGISEQ-500
SRX22328661
GSM7876400_r1
GSM7876400: N2_AbaPep#07 [HaliPep07]; Caenorhabditis elegans; RNA-Seq
SRP469661
PRJNA1034565
SRS19378688
GSM7876400
GSM7876400
RNA-Seq
TRANSCRIPTOMIC
cDNA
Total RNA was extracted from whole nematodes using TRIzol kit (Invitrogen). Oligo(dT)-attached magnetic beads were used to purified mRNA. Purified mRNA was fragmented into small pieces with fragment buffer at appropriate temperature. Then first-strand cDNA was generated using random hexamer-primed reverse transcription, followed by a second-strand cDNA synthesis. Afterwards, A-Tailing Mix and RNA Index Adapters were added by incubating to end repair. The cDNA fragments obtained from previous step were amplified by PCR, and products were purified by Ampure XP Beads, then dissolved in EB solution. The product was validated on the Agilent Technologies 2100 bioanalyzer for quality control. The double stranded PCR products from previous step were heated denatured and circularized by the splint oligo sequence to get the final library. The single strand circle DNA was formatted as the final library. The final library was amplified with phi29 to make DNA nanoball which had more than 300 copies of one molecular, DNBs were loaded into the patterned nanoarray and pair end 100 bases reads were generated on BGIseq500 platform (BGI-Shenzhen, China).
BGISEQ-500