Author: Goodman, Laura B.; Anderson, Renee R.; Slater, Marcia; Ortenberg, Elen; Renshaw, Randall W.; Chilson, Brittany D.; Laverack, Melissa A.; Beeby, John S.; Dubovi, Edward J.; Glaser, Amy L.
Title: High-throughput Detection of Respiratory Pathogens in Animal Specimens by Nanoscale PCR Document date: 2016_11_28
ID: rd1bxkbu_5
Snippet: 1. Use primer design software to verify that each assay conforms to standard probe-based real-time PCR cycling conditions with 60 °C annealing using the primer probe test tool (select the quantification probe setting with default parameters). NOTE: The representative RNA target used was adapted from the universal influenza A matrix targeted assay published by Shu et al. 7 . The primers and probe are as follows: Forward primer: GACCRATCCTGTCACCTC.....
Document: 1. Use primer design software to verify that each assay conforms to standard probe-based real-time PCR cycling conditions with 60 °C annealing using the primer probe test tool (select the quantification probe setting with default parameters). NOTE: The representative RNA target used was adapted from the universal influenza A matrix targeted assay published by Shu et al. 7 . The primers and probe are as follows: Forward primer: GACCRATCCTGTCACCTCTGAC, Reverse Primer: AGGGCATTYTGGACAAAKCGTCTA, Probe: Fam-TGCAGTCCTCGCTCACTGGGCACG-QSY. The representative DNA assay used here was adapted from the equine herpesvirus type 1 (EHV-1) detection method published by Elia et al. 8 . The primers and probe are as follows: Forward primer: GCTCTCAGGTTTTACGACATC, Reverse Primer: CTTTACCCAGGCCCTTGAAA, Probe: FAM-TCAACGTGGACAATACCGCAGTGATTAT-QSY. 2. Order nanoscale PCR amplification plates in the desired configuration.
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