Twist Bioscience NGS | Reagents & Kits | Universal Blockers

The robust design of Twist Universal Blockers maximizes flexibility for a more efficient target enrichment workflow. Compatible with all Twist Target Enrichment Panels, they improve capture of on-target reads independent of index sequence type, across singleplex and multiplex target enrichment workflows, and regardless of panel size. Twist Universal Blockers allow you the flexibility to choose the best adapter index design for your experiment without penalty to target enrichment performance.

Performance is independent of index design. On-target performance of Twist Universal Blockers across a variety of single and dual index TruSeq- compatible adapters. Individual libraries were generated from a single genomic source (NA12878; Coriell) and TruSeq-compatible adapters with index lengths ranging from 6 to 14 bp (unique molecular identifier [UMI] length not included). Hybrid capture was performed either in the absence or presence of Twist Universal Blockers using an exome target enrichment panel (33.1 Mb; Twist Bioscience) using 500 ng of gDNA per individual library following the manufacturer’s recommendations for 16-hour hybridization reactions. Cot DNA was present in all samples. Sequencing was performed with a NextSeq 500/550 High Output v2 kit to generate 2x76 paired end reads. Data was downsampled to 150x of target size and analyzed using Picard Metrics with a mapping quality of 20. Percentage of Bases On-Bait includes both On-Bait and Near-Bait Bases and is defined by the equation 1 - PCT_OFF_BAIT. Error bars denote one standard deviation or range of observations; N ≥ 2.

Performance is independent of panel size. On-target performance of Twist Universal Blockers across a variety of panel sizes. Individual libraries were generated from a single genomic source (NA12878; Coriell) and 8 bp dual-indexed TruSeq-compatible adapters. Hybrid capture was performed either in the absence or presence of Twist Universal Blockers with target enrichment panels of various sizes (0.04Mb to 33.1Mb; Twist Bioscience) and 500 ng of gDNA per individual library following the manufacturer’s recommendations for 16-hour hybridization reactions. Cot DNA was present in all samples. Sequencing was performed with a NextSeq 500/550 High Output v2 kit to generate 2x76 paired end reads. Data was downsampled to 150x of target size and analyzed using Picard Metrics with a mapping quality of 20. Percentage of Bases On-Bait includes both On-Bait and Near-Bait Bases and is defined by the equation 1 - PCT_OFF_BAIT. Error bars denote range of observations; N = 2.