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Plasmids and DNA Constructs¡ªRat DGK-IV cDNA was a generous
gift of K. Goto (Yamagata University School of Medicine, Sendai, Japan).
pSREflagDGKIV was excised with EcoRI, and the 3.4-kb fragment
encoding the DGK-IV cDNA was subcloned in the pcDNA3Myc
vector (pCDNAMycDGK-IV). For expression experiments, all constructs
were subcloned in the pEGFPBos vector in the GFP C terminus.
For the MCA construct, pCDNA3MycDGKIV was digested with BstXI/BglII, and the 2.2-kb fragment was subcloned in pEGFPBos. To generate
the ankyrin domains deletion (ANK), pCMV3MycDGKIV was
SacI-digested, blunted, KpnI-digested, and subcloned in pEGFPBos
digested with KpnI/SmaI. Site-directed mutagenesis was performed
using the QuikChange site-directed mutagenesis kit (Stratagene). To
generate the kinase-dead version of the enzyme, Gly-354 was replaced
with Asp as described (25). We designed two mutations in the MARCKS
homology domain; in the first we replaced Ser-259, Ser-266, Ser-271,
and Ser-272 with Ala (mutant Ser 3 Ala), and in the second the same
residues were replaced with Asp (mutant Ser 3 Asp). To mutate the
CRDs, the first conserved His in each of the two CRDs of the protein,
His-98 or His-173, were replaced with Gly either in the wild type
protein or in the Ser 3 Asp mutant. The C-terminal domain (CT)
construct, including the four ankyrin repeats and the PDZ-binding
motif, was generated by PCR with appropriate primers, which included
two restriction sites, SalI and XbaI. The PCR product was subcloned in
the pGEM-T easy vector (Promega) and then excised with SalI/XbaI to
be subcloned in the expression vector pEFBosCX-HA, which was previously
digested with SalI/XbaI.
Cell Lines and Transient Transfections¡ªCOS-7 cells were maintained
in Dulbecco¡¯s modified Eagle¡¯s medium supplemented with 10%
fetal bovine serum and 2 mM glutamine. For transfection, 60¨C80%
confluent cells were transfected with LipofectAMINE (Invitrogen) according to the manufacturer¡¯s instructions. After 24 h cells were harvested,
and each sample was divided into two pellets for immunoblot
and a DAG activity assay. The J-HM1-2.2 cell line was generated by
stable transfection of the human muscarinic subtype 1 receptor in the
Jurkat cell line (29). Cells were maintained in RPMI 1640 medium
supplemented with 10% fetal bovine serum and 2 mM glutamine. Cells
(1.2  107) were transfected by electroporation with 20 g of DNA using
a Gene Pulser (Bio-Rad) at 270 V and a capacitance of 975 microfarads.
Cells were immediately transferred to 30 ml of growth medium and
assayed 24 h later.

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