Table 2 of Chen, Mol Vis 2010; 16:2016-2025.

Table 2. Primer sequences and PCR conditions for SPARC sequencing.

  Primer sequence      

Amplifying target
Forward primer (5′→3′)
Reverse primer (5′→3′)		 MgCl2
(mM)		 Ta
(°C)		 Size
(bp)
SPARC-1 (promoter + exon 1) CCAGTTCCAAATCATCAAGGA GGGGTTGGTGCAACTATAGAA 1.5 59 668
SPARC-2 (exon 2) AAATGGAACCAACCTCCTCA CAATGGTCCTCATCCCAGTT 1.5 60 388
SPARC-3 (exon 3) AGCTCCCCTAGCCTGTATCC CCCTAATTTCTCAGGGCACA 1.5 60 225
SPARC-4 (exon 4) CTTTCCCTAACACCCCTGGT TCATGTAGGCTGTCCTCGTG 1.5 60 367
SPARC-5 (exon 5) TGTGCTAGTCCAGGTGATGC TGTATTCCGAAGTGCCCAAT 1.5 60 222
SPARC-6 (exon 6) CAGTGTCCCCATCTCTGAAA CCCAAGACAGGAGTCTGGAA 1.5 60 250
SPARC-7 (exon 7) AAGAAACTGTGGCCTGGAGA CTGGTGCTCAGGGGTAAATG 1.5 60 396
SPARC-8 (exon 8) CTGGCTAGTCTCTGCCTGCT TCACTCTAGGGTCTGGGGTCT 2.0 60 279
SPARC-9 (exon 9) GGGTGTGGAGCTTTTCCAT CCCCTTGCTTCTTTGTTCAG 1.5 60 229
SPARC-10 (exon 10) TCCACTGACTCCTTGGGAAG GGCAGAACAACAAACCATCC 1.5 60 198

The promoter (−1 to −318 bp from the transcription initiation site), 5′-untranslated region (the noncoding exon 1), coding regions, exon-intron boundaries, and a portion of the 3′-untranslated region (+1 to +94 bp downstream the stop codon) were covered by the amplimers. In the table, Ta indicates annealing temperature and Bp indicates base pairs.

Chen, Mol Vis 2010; 16:2016-2025. http://www.molvis.org/molvis/v16/a217

©2010 Molecular Vision http://www.molvis.org/molvis/

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