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NEB/NEBNext? Multiplex Oligos for Illumina? (96 Unique Dual Index Primer Pairs)/384 reactions/E6440L
  • NEB/NEBNext? Multiplex Oligos for Illumina? (96 Unique Dual Index Primer Pairs)/384 reactions/E6440L

NEB/NEBNext? Multiplex Oligos for Illumina? (96 Unique Dual Index Primer Pairs)/384 reactions/E6440L

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貨號: E6440L
品牌: NEB
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    • Incorporating a novel hairpin loop structure, the NEBNext® Adaptor ligates with increased efficiency to end-repaired, dA-tailed DNA. The loop contains a U, which is removed by treatment with USER® Enzyme (a mix of UDG and Endo VIII), to open up the loop and make it available as a substrate for PCR. During PCR, barcodes can be incorporated by use of the NEBNext index primers, thereby enabling multiplexing. This kit includes 96 pre-mixed unique pairs of i5 and i7 index primers, packaged in a single-use 96-well plate with a pierceable foil seal.NEBNext Oligos can be used with NEBNext products, and with other standard Illumina-compatible library preparation protocols.Additional dual barcode options (NEB #E7600, NEB #E7780), and single primer options are also available, in 12- and 96- index formats (NEB #E7335, NEB #E7500, NEB #E7710, NEB #E7730, NEB #E6609). A methylated version of the NEBNext Adaptor is also available for use with bisulfite sequencing protocols (NEB #E7535).

      Workflow:

      Designed for use in library prep for DNA, ChIP DNA and RNA (but not Small RNA), the NEBNext Adaptors enable high-efficiency adaptor ligation and high library yields, with minimized adaptor-dimer formation. Incorporating a novel hairpin loop structure, the NEBNext Adaptor ligates with increased efficiency to end-repaired, dA-tailed DNA. The loop contains a U, which is removed by treatment with USER Enzyme (a combination of UDG and Endo VIII), to open up the loop and make it available as a substrate for PCR. During PCR, barcodes can be incorporated by use of the NEBNext index primers, thereby enabling multiplexing. The 96 8-base index primer pairs included in this kit are pre-mixed and are packaged in a single-use 96-well plate with a pierceable foil seal.

      For multiplexing with 384 indices, combine this set with NEB #E6442, NEB #E6444, and NEB #E6446.

      Figure 1: Workflow demonstrating the use of NEBNext Multiplex Oligos for Illumina (96 Unique Dual Index Primer Pairs)

      Figure 2: Use of NEBNext Adaptor and Unique Dual Index Primer Pairs substantially increases library yields and minimizes adaptor-dimers
      16 libraries were prepared with 100 ng of Human NA19240 genomic DNA (Coriell Institute), using the NEBNext Ultra II FS DNA library prep kit. Adaptors and primers were from either the IDT® for Illumina® –TruSeq® DNA UD Indexes (Illumina # 20022370), or the NEBNext Multiplex Oligos for Illumina (96 Unique Dual Index Primer Pairs). After 4 PCR cycles, libraries were quantified on an Agilent® TapeStation® 4000. A) Average library yields for the 8 libraries made using each workflow show 60% higher yield when the NEBNext Adaptor and Unique Dual Index Primer Pairs are used. B) TapeStation traces of 16 libraries show the presence of adaptor-dimer (indicated by the orange arrow) with the libraries made using IDT for Illumina adaptors and primers, which is absent in the libraries prepared using NEBNext adaptors and primers, which also have higher yields.

      Figure 3: Libraries amplified with NEBNext 96 Unique Dual Index Primer Pairs cluster evenly on the Illumina®NovaSeq™ 6000
      96 libraries produced using the NEBNext Ultra II FS DNA library prep kit (Figure 1) and the NEBNext 96 Unique Dual Index Primer Pairs were pooled at equimolar concentrations and sequenced on the Illumina NovaSeq 6000 instrument (2 x 150 bp). The total number of reads from all libraries were summed, and the fraction of the total reads contributed by each library was determined (expected fraction per library=1.04%). All 96 libraries clustered efficiently and were represented at approximately the expected frequency.

      Figure 4: NEBNext 96 Unique Dual Index Primer Pairs amplify libraries with equal efficiency
      Human NA19240 genomic DNA (Coriell Institute) was used to prepare 96 libraries using either the NEBNext Ultra II FS DNA library prep kit, Covaris-sheared DNA with the NEBNext Ultra II DNA library prep kit, the Ultra II DNA library prep kit combined with bisulfite conversion, or the NEBNext Ultra II Directional RNA library prep kit. Libraries were PCR-amplified using the NEBNext 96 Unique Dual Index Primer Pairs to produce libraries containing unique i5 and i7 indices. Library yields were quantified (Agilent®TapeStation®4200) and normalized by summing the total yield of all 96 libraries and calculating the contribution from each library (expected fraction per library = 1.04%). Library amplification efficiency was robust with each library prep method and efficiency was uniform across all 96 unique index primer combinations. Each bar represents the average of at least 2 technical replicates.

      Figure 5: Unique Dual Index Primer Pairs allow identification and discarding of index-hopped reads.
      One set of the 96 NEBNext Ultra II FS DNA libraries (Figure 2) was used to assess the accuracy of read classification and filtering of barcode-hopped reads using unique dual indices. The 96 libraries were pooled at equimolar concentration and the pool was sequenced on both the NovaSeq 6000 (2x150 bp) and MiSeq® (2 x 76 bp) instruments. Reads were demultiplexed using the Picard ExtractIlluminaBarcodes tools considering both indices, and classified into the following categories:
      • Demultiplexed reads: expected i5 and i7 barcode combination
      • Identified index hopping: expected barcodes, but not in expected combination
      • Dark clusters: N or G reads (not observed on MiSeq due to 4-color chemistry)
      • Phi X: any reads matching the universal primer sequence (not present in MiSeq experiment)
      • Other: any remaining reads not fitting into the above categories
      Demultiplexing with a single i5 or i7 index (or a non-unique combination of i5 and i7) incorrectly assigns ~5% of reads on the NovaSeq and 0.6% of reads on the MiSeq, leading to misassignment of reads between samples and problems for downstream analyses. Unique dual indices successfully identify and enable rejection of reads of unknown provenance during demultiplexing.
      Figure 6: Libraries amplified with 384 primer pairs from NEBNext Multiplex Oligos for Illumina (96 Unique Dual Index Primer Pairs Set 1-4) cluster evenly on the Illumina NovaSeq™ 6000
      384 libraries produced using the NEBNext Ultra II DNA Library Prep Kit (NEB #E7645) and the NEBNext Multiplex Oligos for Illumina (96 Unique Dual Index Primer Pairs Set 1-4) were pooled at equimolar concentrations and sequenced on the Illumina NovaSeq® 6000 instrument. The total number of reads from all libraries were summed, and the fraction of the total reads contributed by each library was determined (expected fraction per library = 0.26 %). All 384 libraries clustered efficiently and were represented at approximately the expected frequency.
      This product is related to the following categories:
      NEBNext? Multiplex Oligos (Adaptors & Primers),
      Next Generation Sequencing Library Preparation
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