PHOSPHORYLATION BY PROTEIN-KINASE-A OF RCK1 K+ CHANNELS EXPRESSED IN XENOPUS-OOCYTES

被引：63

作者：

IVANINA, T

PERETS, T

THORNHILL, WB

LEVIN, G

DASCAL, N

LOTAN, I

机构：

[1] TEL AVIV UNIV,SACKLER SCH MED,DEPT PHYSIOL & PHARMACOL,IL-69978 RAMAT AVIV,ISRAEL

[2] MT SINAI HOSP,MT SINAI SCH MED,DEPT PHYSIOL & BIOPHYS,NEW YORK,NY 10029

来源：

BIOCHEMISTRY | 1994年 / 33卷 / 29期

关键词：

D O I：

10.1021/bi00195a021

中图分类号：

Q5 [生物化学]; Q7 [分子生物学];

学科分类号：

071010 ; 081704 ;

摘要：

Phosphorylation-mediated regulation of voltage-gated K+ channels has been implicated in numerous electrophysiological studies; however, complementary biochemical studies have so far been hampered by the failure to isolate and characterize any K+ channel proteins of distinct molecular identity. We used the Xenopus oocyte expression system to study the biosynthesis and phosphorylation by protein kinase A (PKA) of rat brain RCK1 (Kv1.1) K-+ channel protein. RCK1 protein was isolated by immunoprecipitation from oocytes injected with RCK1 cRNA and analyzed by SDS-polyacrylamide gel electrophoresis (SDSPAGE). The channel protein was expressed in the form of several polypeptides. The 57-kDa polypeptide, usually the major constituent, resided both in the cytosol and in the plasma membrane. Its levels were correlated with RCK1 current amplitudes (I-RCK1) and upon incubation of the cRNA-injected oocytes with tunicamycin, its molecular weight was decreased and at the same time I-RCK1 was reduced. These results suggest that the membranal 57-kDa polypeptides represent functional channels that are N-glycosylated. Furthermore, a study of the phosphorylation of the RCK1 polypeptides revealed that the 57-kDa polypeptide was specifically targeted for phosphorylation by PKA. It could be phosphorylated in vitro by the catalytic subunit of PKA (PKA-CS). In its native state in intact oocytes, the 57-kDa polypeptide was partially phosphorylated and could be further phosphorylated in vivo by addition of a membrane-permeant cAMP analog. Site-directed mutagenesis demonstrated that phosphorylation of a single site on the C-terminus of the channel molecule fully accounts for these phosphorylations. This work thus characterizes biochemically what appears to be a functional K-+ channel polypeptide, demonstrates its phosphorylation by PKA in vitro and in intact cells, and localizes the phosphorylation site on the molecule.

引用

页码：8786 / 8792

页数：7

共 40 条

[1] EFFECTS OF MODULATORS OF ADENYLYL CYCLASE ON INTERLEUKIN-2 PRODUCTION, CYTOSOLIC CA-2+ ELEVATION, AND K+ CHANNEL ACTIVITY IN JURKAT T-CELLS
BASTIN, B
PAYET, MD
DUPUIS, G
[J]. CELLULAR IMMUNOLOGY, 1990, 128 (02) : 385 - 399
[2] STRUCTURE OF THE VOLTAGE-DEPENDENT POTASSIUM CHANNEL IS HIGHLY CONSERVED FROM DROSOPHILA TO VERTEBRATE CENTRAL NERVOUS SYSTEMS
BAUMANN, A
GRUPE, A
ACKERMANN, A
PONGS, O
[J]. EMBO JOURNAL, 1988, 7 (08) : 2457 - 2463
[3] SINGLE CARDIAC OUTWARDLY RECTIFYING K+ CHANNELS MODULATED BY PROTEIN KINASE-A AND A G-PROTEIN
BENZ, I
FROBE, U
KOHLHARDT, M
[J]. EUROPEAN BIOPHYSICS JOURNAL WITH BIOPHYSICS LETTERS, 1991, 20 (05): : 281 - 286
[4] SOLUBILIZATION AND PHYSICAL CHARACTERIZATION OF ACCEPTORS FOR DENDROTOXIN AND BETA-BUNGAROTOXIN FROM SYNAPTIC-MEMBRANES OF RAT-BRAIN
BLACK, AR
DONEGAN, CM
DENNY, BJ
DOLLY, JO
[J]. BIOCHEMISTRY, 1988, 27 (18) : 6814 - 6820
[5] BLUMENTHAL EM, 1992, J NEUROSCI, V12, P290
[6] AN AMINO-ACID MUTATION IN A POTASSIUM CHANNEL THAT PREVENTS INHIBITION BY PROTEIN-KINASE-C
BUSCH, AE
VARNUM, MD
NORTH, RA
ADELMAN, JP
[J]. SCIENCE, 1992, 255 (5052) : 1705 - 1707
[7] CAI YC, 1993, J BIOL CHEM, V268, P23720
[8] TOXINS IN THE CHARACTERIZATION OF POTASSIUM CHANNELS
CASTLE, NA
HAYLETT, DG
JENKINSON, DH
[J]. TRENDS IN NEUROSCIENCES, 1989, 12 (02) : 59 - 65
[9] Dascal N., 1992, METHODS MOL BIOL VOL, VVolume 13, P205
[10] DREWE JA, 1992, J NEUROSCI, V12, P538

← 1 2 3 4 →