Table 1 of Kim, Mol Vis 2009; 15:833-843.

Table 1. Primers for the RS1 mutation analysis.

Gene Usage Exon Primer (5′→3′)
RS1 PCR and sequencing 1 F: GGTTAACTTGATGGGGCTCA
R: CCCATCCTGTTTTCTGTTGG
2 F: TTCTTCCAGAAGGGGTGTTG
R: AAGCGATTCTCTTGCCTCAG
3 F: TCAATTTGGCCATTGTAGCA
R: GGAGAAAACCCGCATTAACA
4 F: TGAACCGTTGAAGACACAGC
R: AGTGCAGTGGTGTGATCTCG
5 F: TTTCTTGGGAGGTGGAGATG
R: GCAGATGATCCACTGTGCTG
6 F: GTTCCAGATGTCCCAAGCAT
R: TGCGAAATATAGCCCTGTCC
RS1 Gene dosage 1 F: GGGAAGATGTCACGCAAGAT
R: AACTGGAAAGCCATCCACAC
2 F: GCCACATTGGGATTATCGTC
R: TGTTGGGATTACAGGCATGA
3 F: AACCACAGTTGCCTTTGACC
R: TGTTCCCAATGACTGTTCCA
4 F: CAGTCACCTGGTGCTTGTTG
R: CGAAGAATACCAGCCCACAT
5 F: TTTCTTGGGAGGTGGAGATG
R: TGTCCTGGAACTTGGAGAGC
6 F: GTTCCAGATGTCCCAAGCAT
R: GGTCCGAGTTGCCATAGAAG
HBB Gene dosage 2 F: TTGGACCCAGAGGTTCTTTG
R: GAGCCAGGCCATCACTAAAG
B2M Gene dosage 2 F: CTCACGTCATCCAGCAGAGA
R: AGTGGGGGTGAATTCAGTGT

Forward and reverse primers sequences were used to amplify the RS1, HBB, and B2M genes. Forward primers for gene dosage analysis were labeled with 6-FAM. Annealing temperature was 55 °C, with exception of RS1 primers for amplification of exon 2 (60 °C), exon 4 (60 °C), and exon 5 (58 °C).

Kim, Mol Vis 2009; 15:833-843. http://www.molvis.org/molvis/v15/a86

©2009 Molecular Vision http://www.molvis.org/molvis/

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