TABLE 3.
Primers used for site-directed mutagenesis and reverse PCRs in this study
| Description/function | Primer sequence (5′–3′) | Source |
|---|---|---|
| Introduction of a K165R mutation into LpdA by site-directed mutagenesis PCR | ATAATTCGATTGCGTCCAACCATAATAGAGCCATCTGGATTG | This study |
| CAATCCAGATGGCTCTATTATGGTTGGACGCAATCGAATTAT | ||
| Introduction of a K376R mutation into LpdA by site-directed mutagenesis PCR | GAAAAAAGAGGTTATTCATATGAGATTTATGTCAATTGATGGGCAGG | This study |
| CCTGCCCATCAATTGACATAAATCTCATATGAATAACCTCTTTTTTC | ||
| Fusion of a calreticulin ER retention signal to mCherry by reverse PCR | GAGCAGCAGCGGCACGGATAGCAGCATGGTGGCGACCGGTAGGG-CCTTCTTGGCCTAGCAGT | This study |
| AGCAGTGAGCAAGGGCGAGGAG | ||
| Fusion of a KDEL ER targeting signal to mCherry by reverse PCR | GAGCTGTAACTGATCATAATCAGCCATACC | This study |
| ATCCTTTCTAGATCCGGTGGATCCC |