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A rapid method for detecting specific amplified PCR fragments in microtiter plates.

Nucleic acids research (1996-08-15)
A Ortiz, E Ritter
ZUSAMMENFASSUNG

A simple method is presented to circumvent laborious and time consuming electrophoretic separations of specific PCR amplification products. Specific target DNA is amplified using nucleotides labelled with DIG-dUTP or biotin-dCTP. The labelled PCR products are separated from unincorporated nucleotides or oligonucleotides by using a positively charged DEAE cellulose matrix. Amplification products are visualized directly in the matrix using immunoenzymatic methods or streptavidin-conjugated enzymes. The detection process can be carried out within 2 h, allows the processing of large sample sizes and can potentially be automated.

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Sigma-Aldrich
Diethylaminoethyl–Sephacel®, aqueous ethanol suspension, 40-160 μm (wet), exclusion limit ~1,000,000 Da