Ha ubiquitin k63

PCR-amplified human p62 was cloned into pcDNA3.1/hygro(+)-Flag, pcDNA3-HA, or pColdI (His) vector. Human AMPKα1 was cloned into pcDNA3-HA vector. The construction of Flag/V5–rKHK-A or Flag/V5–rKHK-C, GST–KHK-A or GST–KHK-C, Flag-rKHK G257R, His-PRPS1, and KHK short hairpin RNA (shRNA) was described previously (32 (link)). Nrf2 CA (with the deletion of amino acids 1 to 89) was cloned into pcDNA3.1/puro(+)-HA. PINK1 and SQSTM1 shRNA were constructed via ligation of an oligonucleotide targeting human PINK1 (5′-GCTGGAGGAGTATCTGATAGG-3′) and p62 (5′-ACTGGACCCATCTGTCTTCAA-3′) into an Xho I–/Mlu I–digested pGIPZ vector, respectively. Flag-, V5-, or GST-tagged rKHK-A S80A, Flag–rKHK-A S80E, Flag-p62 S28E, Flag-p62 S28A, His–p62 S28A, Flag–p62 K7R, and all the shRNA-resistant p62 constructs containing nonsense mutations of C1017T, T1020C, and G1023A were constructed using the QuikChange Site-Directed Mutagenesis Kit (Stratagene, La Jolla, CA). Vectors expressing GFP-LC3, HA-ubiquitin-WT, HA-ubiquitin-K48, and HA-ubiquitin-K63 were purchased from Addgene.