Home Failure Case Library Few or No Transformants After Cloning
Restriction Enzyme Digest severe

Few or No Transformants After Cloning

Symptom
Bacterial transformation yields few or no colonies after restriction digest-based cloning. Vector may not be linearized or insert ends incompatible.
Common Causes
  1. 1 Recognition site blocked by Dam, Dcm, or CpG methylation preventing cleavage
  2. 2 Incorrect buffer used reducing enzyme activity to <10%
  3. 3 DNA contaminants (salts, proteins, polysaccharides) inhibiting enzyme
  4. 4 PCR fragment has <6 nucleotides between recognition site and DNA end, preventing cleavage
Solutions
  1. 1 Check enzyme methylation sensitivity; use dam⁻/dcm⁻ strain (NEB #C2925) for methylation-sensitive enzymes
  2. 2 Use recommended NEBuffer supplied with restriction enzyme; verify 100% activity
  3. 3 Clean up DNA with spin column (NEB #T1030) to remove inhibitors before digestion
  4. 4 Design PCR primers with ≥6 nucleotides flanking the recognition site at DNA ends
Related Video (3)
New England Biolabs ★ 92
Cloning With Restriction Enzymes
"Directly addresses restriction enzyme selection and usage in cloning workflows, essential for understanding proper digest conditions and potential failure points"
Addgene ★ 78
Restriction Digest Analysis
"Demonstrates restriction digest analysis including gel identification of band patterns, helping researchers verify whether linearization occurred and diagnose incomplete digestion"
New England Biolabs ★ 72
How to Perform a Transformation with NEB Competent Cells
"Covers transformation protocol with competent cells, providing context for the downstream step where few/no colonies would be observed as the symptom of upstream cloning failure"
Source: neb.com ↗
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