Table 1 of Chen, Mol Vis 2014; 20:132-139.

Table 1. Primers used in sequencing of the RS1 gene and allele-specific PCR analysis.

Exon/mutation site Primer sequence (5′-3′) Size (bp) TM (°C)
1 F:TCTTCCATGAGACTTCCTTGTTGA 485 60
R:AGATTTCTGAGACCCATCCTGTT
2 F:TCTTCCATGAGACTTCCTTGTTGA 249 58
R:TACATTTAAAAACAAAGTGATAGTCCTC
3 F:CCAGGGTGGCAGACATTTT 406 60
R:GGTAGCGTTCAGGGGGTT
4 F:TTCCTTTACTTCATCCTTCATTCC 550 60
R:CTCACTGTAACCTCCGCTTCC
5 F:GCAGGGAGAGGGAGAATGAGA 570 60
R:CCAAAGCAAGCCCAGGAA
6 F:CAGTTCCAGATGTCCCAAGCA 432 62
R:TGTCCATCTCGGTGGTGTGTG
5/p.Y151H R: TCCTGTACTGCACGCTGaG 347 60
5/p.Y166H R:TTCCAGTCTGGTCCTTGaG 392 60
5/p.K167E R:GTTGTTTCCAGTCTGGTCCaC 397 60
6/p.I194N R:CGGATGAAGCGGGAGATGT 271 62

Abbreviations: F: forward; R: reverse; primer sequences with lower case indicate modified nucleotides to specifically amplify the mutant sequence; red, mutation-specific nucleotide.

Chen, Mol Vis 2014; 20:132-139. http://www.molvis.org/molvis/v20/132

©2014 Molecular Vision http://www.molvis.org/molvis/

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