Table 1 of Wang, Mol Vis 2009; 15:181-186.

Table 1. Primers used for polymerase chain reaction amplification and sequencing of MFRP.




Exon


Primer sequence (5'-3')		 Size of
PCR
product
(bp)
Annealing
temperature
(°C)


Note
1,2 F-CTTTTCCCTCGGGTAGTAGA 466 60 GC buffer
R-GTTGGCAGGTGGGGTTTTGAA


3,4 F-AGGACAGCATGAGGAATACC 504 62
R-AACCCCACCCCGTCATCTTG


5 F-GAGAAGGGCCCAAGATGACG 405 63 GC buffer
R-TCCCTGCCACTCCCTGATTC


6,7 F-TTGGGGGTTGAGAAAATAGG 601 58
R-CTGGGCCAAAGAATGACTGA


8 F-ATCACCGCCAGCCCTATTG 281 62
R-CATCCCCCGTCTGCTTGAT


9 F-GGTGCCCGGGATGAGACAG 267 62 GC buffer
R-CCGGGGGTGGCAGACAGT


10,11 F-GCAGTGCCCCCTCAGTCAGC 511 64
R-GTGGGCACCCAGCCTGCTC


12,13 F-CAGGCCACAGAGCCAGTGAG 548 63
R-AGCCCTGACCGGCAAAAGAG


GC buffer was provided by Takara Biotechnology (Dalian) CO.Ltd (Liaoning,China) and designed for amplification of templates having complex secondary structure or high GC content. In the "Primer sequence" column, "F" indicates the forward sequence and "R" indicates the reverse sequence.

Wang, Mol Vis 2009; 15:181-186. http://www.molvis.org/molvis/v15/a17

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

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