Home Genetics / Genomics Best Practices for Nextera Library Prep Expert Video Tip
Steps
  1. 1 Assess sample quality and quantity 00:38
  2. 2 Perform tagmentation reaction 00:38
  3. 3 Understand under-tagmentation causes and prevention 01:46
  4. 4 Understand over-tagmentation causes and prevention 03:37
  5. 5 Perform quality control checks on libraries 05:36
  6. 6 Quantify final library using appropriate method 06:41
  7. 7 Normalize and prepare libraries for sequencing 07:41
  8. 8 Access support resources and troubleshooting guides 08:50
Genetics / Genomics Illumina

Best Practices for Nextera Library Prep Expert Video Tip

Protocol
Difficulty
intermediate

Steps

1
Assess sample quality and quantity

Evaluate the quality and quantity of input DNA using fluorometric methods like Qubit or Picogreen, avoiding UV absorbance. Check purity ratios (260/280 >1.8 and 280/230 >2.0) and perform additional purification if needed to remove contaminants.

▶ 00:38
2
Perform tagmentation reaction

Incubate DNA with the modified transposon to simultaneously cleave and tag the DNA with partial adapter sequences. Ensure accurate DNA input to avoid under-tagmentation (too much DNA) or over-tagmentation (too little DNA).

▶ 00:38
3
Understand under-tagmentation causes and prevention

Learn how excess DNA input or enzymatic inhibitors (EDTA, proteins, detergents, phenols) lead to under-tagmentation and inefficient clustering. Use proper quantification and purification methods to prevent larger-than-optimal library fragments.

▶ 01:46
4
Understand over-tagmentation causes and prevention

Identify three main causes of over-tagmentation: insufficient DNA input, degraded DNA (FFPE samples), and small amplicons. For amplicon libraries, use DNA fragments at least 300 base pairs with primers designed 50+ base pairs upstream and downstream.

▶ 03:37
5
Perform quality control checks on libraries

Run tagmented samples on a high sensitivity bioanalyzer to verify library size distribution (200 base pair to 1.5 KB). Optionally run samples after PCR amplification before bead cleanup to confirm fragments exceed 200 base pairs.

▶ 05:36
6
Quantify final library using appropriate method

Use fluorometric methods (Qubit or Picogreen) to quantify double-stranded DNA after PCR cleanup. Do not use bioanalyzer traces or qPCR for quantification due to broad library distribution.

▶ 06:41
7
Normalize and prepare libraries for sequencing

For Nextera XT kits, use bead-based normalization by adding libraries to normalization beads; elute normalized single-stranded libraries that can be pooled at 1:1 volume ratio. Store double-stranded libraries frozen before normalization, and keep single-stranded libraries at -20°C for up to one week.

▶ 07:41
8
Access support resources and troubleshooting guides

Consult Illumina's technical support pages, troubleshooting technical notes, and field application scientists for additional guidance on Nextera library preparations.

▶ 08:50
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