Table 2. Analysis of DNA and RNA: Primers in relation to assays used in the study.
| Size | Gene | Amplification Primers (5′ - 3′) | Sequencing Primers (5′ - 3′) | *Modified Sequence/corresponding unmodified sequence analyzed (5′ - 3′) | |
|---|---|---|---|---|---|
| Q-PCR | 346 bp | ITGA9-F | CCCCGCTGACTCGTTCTT | ||
| ITGA9-R | TAGGATGTGGTCGGCTTC | ||||
| 487 bp | WNT7A-F | GGGACTATGAACCGGAAAGC | |||
| WNT7A-R | CGATGCCGTAGCGGATGT | ||||
| 67 bp | GAPDH-F | AGCCACATCGCTCAGACAC | |||
| GAPDH-R | GCCCAATACGACCAAATCC | ||||
| BS-cloning sequencing | 341 bp | ITGA9-F | TTGAGTGGGATTTGAGGATTTGTAT | ||
| ITGA9-R | ACCTATCTCCCTACCTTTATCTCTCTTTC | ||||
| 683 bp | WNT7A-F | TTTAGGTTGAGAAAGAGGTGGTTTA | |||
| WNT7A-R | AACAAAACAACAAACCAAAACACTA | ||||
| BS-pyrosequencing | ITGA9-S1-F | AGTGGGATTTGAGGATTTGT | AGGATTTGTATTT TTTGATAAG | TTTTTAGATGAYGTTGATGTTGTTGGTTYGGAG ATTATATTTYGGGAATTATTGGTGTAYGAGATTA AGTGATTAGAATATGGAG | |
| ITGA9-S1-R | biotin-CCCTCCATATTCTAATCACTTAAT | TTCCCAGATGACGTTGATGCTGCTGGTCCGGA GACCACACTTCGGGAATCACTGGTGTACGAG ACCAAGTGACTAGAATATGGAG | |||
| ITGA9-S2-F | ATTGGGTGAAGGAGTAGAGGA | GAAGGAGTAGA GGATG | YGTAGGGTTAGAATTTGGAGTTTAAATTYGTT TTTTATTYGGGTTGTTTTGGATTTTATTGGTTG | ||
| ITGA9-S2-R | biotin-CCCTCCCTATCTCACAACCAATAA | CGCAGGGCTAGAACCTGGAGTCTAAACTCGT CCTTCACCCGGGTTGCTCTGGACTTACTGGTTG | |||
| MSP | 230 bp | ITGA9-F | GTTGTTGGTTCGGAGATTATATTTC | ||
| ITGA9-R | AAAACAACCCGAATAAAAAACG | ||||
| 123 bp | WNT7A-F | GTAGTTCGGCGTCGTTTTAC | |||
| WNT7A-R | CGAAACCGTCTATCGATACG | ||||
| 184 bp | β-ACTIN F | AAGTTAAGTTTTGTTTTTATTTTTTTT | |||
| β -ACTIN R | CAATAATCTCCTTCTACATCCTATC |
*
The cells with italic text show the unmodified sequences analyzed by bisulfite pyrosequencing.