Real lab failures, root causes, and fixes — curated and bilingually annotated by our team.
No bands visible on agarose gel after PCR amplification, indicating complete reaction failure.
Extra, unwanted bands appear on gel in addition to or instead of the target product, indicating off-target amplification.
Small molecular weight band (typically 50-100 bp) visible at bottom of gel, representing primer self-amplification artifacts that compete with target amplification.
No amplification product visible despite proper template and reagents, suggesting thermal cycling conditions are inappropriate.
Amplified DNA appears as broad smear rather than discrete bands, indicating degradation or over-amplification artifacts.
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