Bioanalyzer or gel electrophoresis reveals smearing or loss of distinct RNA bands. RNA integrity number (RIN) is significantly reduced compared to input material.
Common Causes
1RNase contamination from lab bench surfaces, gloves, or non-RNase-free plasticware
2Use of non-disposable pipet tips or microfuge tubes that may harbor RNase activity
3Kit components left unsealed or exposed to ambient air during processing
4Improper post-purification storage - RNA stored at temperatures above -70°C or subjected to freeze-thaw cycles
Solutions
1Work on a clean, RNase-free lab bench; wipe surfaces with RNase decontamination solution before use
2Wear powder-free gloves throughout the procedure; change gloves frequently to prevent cross-contamination
3Use only disposable RNase-free pipet tips and microfuge tubes (not provided in kit); avoid autoclaved reusable plasticware
4Keep all kit components tightly sealed when not in use; minimize exposure time during reagent handling
5Use purified RNA immediately in downstream applications or aliquot and store at -70°C; avoid repeated freeze-thaw cycles