Table 2 of Fink, Mol Vis 2008; 14:1737-1751.

Table 2. cDNA PCR primers.



Gene

Target

Primer
Primer
location

Primer sequence (5′-3′)		 Annealing
Temperature
(°C)		 Product
Size
(bp)
TNNT1 cDNA TNNT1ex1–9_F Exon 1 GCCGAAGAGCAAGAATATGA 58 °C 492


TNNT1ex1–9_R Exon 9 GACCAGATAACCCCCAAAAT



TNNT1ex8–13_F Exon 8 GCTTCAGAACCGAGAAGGA 58 °C 533


TNNTex8–13_R Exon 13 CCCAGATGGACACACACC



TNNT_ex4_F_cDNA Exon 1/2 AGAGGAGCAGCCCTGAAGA 60 °C 172


TNNT_ex4_R_cDNA Exon 6 ATGTCATCGAAGTCCACACG

RDH13 cDNA RDH13_cF1 Exon 1 GCGCTCTAGGTGCAGACTCCG 60 °C 714


RDH13_cR1 Exon 5 CTCAGCTCCTTGGTGGAGAC



RDH13_cF2 Exon 3 GAAGTCCATCCGAGAGTTCG 60 °C 789


RDH13_cR2 Exon 7 GGCATGACAGCTAGGTTTGG

TFPT cDNA TFPT_ex1_F Exon 1 GAGCCCGATAAACAGACTCG 60 °C 655


TFPTex1–2_R Exon 3 GCTGGAGTCTCCGAGTTATTC



TFPTex1–2_F Exon 2 GTGGGCTTCGAGGAGTTC 60 °C 689


TFPT_ex6_R Exon 6 TAGGGCAGCAGTTTGTCTGG

The PCR primers for the amplification of the cDNA of bovine TNNT1, RDH13, and TFPT are shown.

Fink, Mol Vis 2008; 14:1737-1751. http://www.molvis.org/molvis/v14/a206

©2008 Molecular Vision http://www.molvis.org/molvis/

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