Abstract
Although myristoylated alanine-rich C kinase substrate (MARCKS), has been employed as an indicator for the activation of protein kinase C (PKC) in intact cells, little is known about its specificity for PKC family members. To address this question, we partially purified human MARCKS from baculovirus-infected cells and compared the kinetic parameters for phosphorylation by PKC isozymes, conventional PKC alpha (cPKC alpha), novel PKC delta (nPKC delta), nPKC epsilon, and atypical PKC zeta (apKC zeta), all of which are distributed in a wide variety of cells. cPKC alpha, nPKC delta, and nPKC epsilon efficiently phosphorylated intact MARCKS protein in vitro. The affinity of MARCKS for cPKC alpha, nPKC delta, and nPKC epsilon was extremely high and decreased in the order alpha > delta > epsilon with Km values of 10.7, 20.7, and 29.8 nM, respectively. The rate of phosphorylation also decreased in the same order. In contrast, a PKC zeta did not phosphorylate MARCKS efficiently, and we were unable to estimate the kinetic parameters. These results suggest that cPKC alpha, nPKC delta, and nPKC epsilon but not a PKC zeta are enzymes that phosphorylate MARCKS in response to PKC activators in intact cells. The structural requirements of MARCKS for efficient phosphorylation by these PKC members were then examined using a peptide that surrounds the phosphorylation site of MARCKS (peptide MARCKS). Interestingly, intact MARCKS showed a 90-150 times lower rate of phosphorylation by PKCs compared with peptide MARCKS, whereas the former showed a 40-180 times higher affinity for these PKC members. This implies that intact MARCKS protein retains a very high affinity for PKC with the sacrifice of its phospho-accepting activity. The structural requirements of PKC were then examined using a calpain-cleaved active fragment of nPKC delta. MARCKS was phosphorylated by the active catalytic fragment as efficiently as by intact nPKC delta, indicating that the kinase domain is sufficient for the high affinity interaction with intact MARCKS. However, gel overlay assay revealed that both intact nPKC delta and its regulatory domain bind to MARCKS, suggesting that both the kinase and regulatory domains of nPKC delta are involved in the high affinity interaction with intact MARCKS protein.
Highlights
The activation of protein kinase C (PKC)in intactcells, little is known about its specificity forPKC family members
We investigate the specificity of Protein kinase C (PKC) members by determining the kinetic constants for conventional PKCa (cPKCa), nPKCS, and aPKCC) werehighlypurified from recombinantbaculovirus-infected St21 cells? In brief, Si21cells were infected witha recombinant PKC virus.Threedaysafterinfection,the cell pelletswere extracted, and thecytoplasmic fractions were purifiedby a series of chromatographic steps including DEAE-cellulose (Tosoh), hydroxyapatite (Koken), andMono Q column chromatographiesfor cPKCa, nPKCS, and nPKCE, and aPKC6 using both partially purified human nPKCE and DEAE-cellulose, heparin (%soh), and phenyl (Pharmacia)
It is evident that a single cell usually contains multiplePKC isozymes including nPKCmembers that are activatedby PKC activators such as TPA
Summary
RQKNV), corresponding to the cPKCa pseudosubstrate site with a n Phosphopeptide Mappingof MARCKS-Peptide mapping by limited alanine to serine substitution, was a gift from Dr Tatsuya Tamaoki, proteolysis in SDS was performedas described previously [44]. Kyowa Hakko Kogyo Co., Ltd. Grace's insect medium, fetal bovine se- MARCKS (12 ng) was phosphorylatedby cPKCa, nPKCS, or nPKCe for rum, and antibiotics were fromLife Technologies, Inc. Medium supple- 30 min as described above. Native MARCKS (80,8, 0.8 ng) was subjected to SDS-PAGE, blotted onto nitrocellulose, and thentreatedwitha 5% skimmilksolution.Thenitrocellulosewas overlaid with lo6cpm of "P-labeled nPKCS diluted in 50mM Tris-HC1, pH 7.5,0.5 M NaCl, 40 pg/ml PS, and 1%bovine serum albuminat room temperature for 5 h. Immunoblot analysis [48] for MARCKS was performed after the overlayassay
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