Table 1 of Asomugha, Mol Vis 2011; 17:2407-2420.

Table 1. Oligonucleotide primers used for subcloning WT αB-crystallin and deamidated αB species, and generating truncated αB mutant proteins using PCR-based deletion.

Mutant constructs Direction Primers (5′–3′)
WT αB forward CACCATGGACATCGCCATCCACCACCCCTG
  reverse CTATTTCTTGGGGGCTGCGGTGACAGC
αB N146D forward CACCATGGACATCGCCATCCACCACCCCTG
  reverse CTATTTCTTGGGGGCTGCGGTGACAGC
αB-NT forward CACCCGCCTGGAAAAGGACAGGTTCTCTG
  reverse CTATTTCTTGGGGGCTGCGGTGACAGC
αBN146D-NT forward CACCCGCCTGGAAAAGGACAGGTTCTCTG
  reverse CTATTTCTTGGGGGCTGCGGTGACAGC
αB-CT forward CACCATGGACATCGCCATCCACCACCCCTG
  reverse TTATTTCCTTGGTCCATTCACAGTGAG
αBN146D-CT forward CACCATGGACATCGCCATCCACCACCCCTG
  reverse TTATTTCCTTGGTCCATTCACAGTGAG

NT and CT denote the NH2-terminally truncated and COOH-terminally truncated mutant proteins, respectively.

Asomugha, Mol Vis 2011; 17:2407-2420. http://www.molvis.org/molvis/v17/a262

©2011 Molecular Vision http://www.molvis.org/molvis/

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