A simplified procedure for developing multiplex PCRs. | Zendy

Anthony P. Shuber | Zendy; Valerie Grondin | Zendy; K. Klinger | Zendy

AI Assistant Blog Pricing

Home ZAIA Blog

Open Access

A simplified procedure for developing multiplex PCRs.

Author(s) -

Anthony P. Shuber,

Valerie Grondin,

K. Klinger

Publication year - 1995

Publication title -

genome research

Language(s) - English

Resource type - Journals

SCImago Journal Rank - 9.556

H-Index - 297

eISSN - 1549-5469

pISSN - 1088-9051

DOI - 10.1101/gr.5.5.488

Subject(s) - primer (cosmetics) , multiplex , multiplex polymerase chain reaction , biology , computational biology , primer dimer , polymerase chain reaction , genetics , microbiology and biotechnology , nucleic acid sequence , multiplex ligation dependent probe amplification , dna , gene , chemistry , organic chemistry , exon

We have developed a simplified method for multiplex PCR based on the use of chimeric primers. Each primer contains a 3' region complementary to sequence-specific recognition sites and a 5' region made up of an unrelated 20-nucleotide sequence. Identical reaction conditions, cycling times, and annealing temperatures have been established for any PCR primer pair comprising the chimeric motif. Under these conditions, efficient multiplex amplification is achieved easily and reproducibly by simple adjustment of the individual primer concentrations. No additional modification of either the reaction components or annealing temperatures is required. The use of tagged primers provides a method for primer design that eliminates the multiple optimization steps involved in developing multiplex PCR.

The content you want is available to Zendy users.

Already have an account? Click here to sign in.

Having issues? You can contact us here

Accelerating Research