Differential regulation of retinoblastoma protein function by specific Cdk phosphorylation sites

被引：279

作者：

Knudsen, ES

Wang, JYJ

机构：

[1] UNIV CALIF SAN DIEGO,DEPT BIOL,LA JOLLA,CA 92093

[2] UNIV CALIF SAN DIEGO,CTR GENET MOLEC,LA JOLLA,CA 92093

来源：

JOURNAL OF BIOLOGICAL CHEMISTRY | 1996年 / 271卷 / 14期

关键词：

D O I：

10.1074/jbc.271.14.8313

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：

The retinoblastoma tumor suppressor protein, RE, contains at least three distinct protein binding domains. The A/B pocket binds proteins with the LXCXE motif, the C pocket binds the nuclear c-Abl tyrosine kinase, and the large A/B pocket binds the transcription factor E2F. Dissociation of RE from its targets is observed as RE becomes phosphorylated during G(1)/S progression. There are 16 Cdk consensus phosphorylation sites in RE. It was previously unknown whether the many phosphorylation sites had redundant or distinct functions in the regulation of RE. Using RE mutant proteins lacking specific phosphorylation sites, we show that each of the binding domains is inhibited by different sites. Thr-821/826 phosphorylation is required to inhibit the binding to LXCXE containing proteins. Mutation of these two sites does not interfere with the hyperphosphorylation of RE. However, this phosphorylated mutant retains the ability to bind T-Ag, E7, and Elf-1, all of which contain the LXCXE motif. In contrast, Ser-807/811 phosphorylation is required to disrupt c-Abl binding. Mutation of Ser-807/811 and Thr-821/826 does not abolish the regulation of E2F binding. Taken together, these results show that the protein binding domains of RE are each regulated by distinct Cdk phosphorylation sites.

引用

页码：8313 / 8320

页数：8

共 29 条

[1] SUPPRESSION OF HUMAN COLORECTAL-CARCINOMA CELL-GROWTH BY WILD-TYPE-P53
BAKER, SJ
MARKOWITZ, S
FEARON, ER
WILLSON, JKV
VOGELSTEIN, B
[J]. SCIENCE, 1990, 249 (4971) : 912 - 915
[2] HIGH-EFFICIENCY TRANSFORMATION OF MAMMALIAN-CELLS BY PLASMID DNA
CHEN, C
OKAYAMA, H
[J]. MOLECULAR AND CELLULAR BIOLOGY, 1987, 7 (08) : 2745 - 2752
[3] THE RETINOBLASTOMA-SUSCEPTIBILITY GENE-PRODUCT BECOMES PHOSPHORYLATED IN MULTIPLE STAGES DURING CELL-CYCLE ENTRY AND PROGRESSION
DECAPRIO, JA
FURUKAWA, Y
AJCHENBAUM, F
GRIFFIN, JD
LIVINGSTON, DM
[J]. PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1992, 89 (05) : 1795 - 1798
[4] ANALYSIS OF ORIGIN OF DNA-REPLICATION OF HUMAN PAPOVAVIRUS BK
DEYERLE, KL
SAJJADI, FG
SUBRAMANI, S
[J]. JOURNAL OF VIROLOGY, 1989, 63 (01) : 356 - 365
[5] FUNCTIONAL INTERACTIONS OF THE RETINOBLASTOMA PROTEIN WITH MAMMALIAN D-TYPE CYCLINS
EWEN, ME
SLUSS, HK
SHERR, CJ
MATSUSHIME, H
KATO, JY
LIVINGSTON, DM
[J]. CELL, 1993, 73 (03) : 487 - 497
[6] THE RETINOBLASTOMA GENE-PRODUCT REGULATES PROGRESSION THROUGH THE G1 PHASE OF THE CELL-CYCLE
GOODRICH, DW
WANG, NP
QIAN, YW
LEE, EYHP
LEE, WH
[J]. CELL, 1991, 67 (02) : 293 - 302
[7] TRANSCRIPTIONAL REPRESSION OF THE E2-CONTAINING PROMOTERS EIIAE, C-MYC, AND RB1 BY THE PRODUCT OF THE RB1 GENE
HAMEL, PA
GILL, RM
PHILLIPS, RA
GALLIE, BL
[J]. MOLECULAR AND CELLULAR BIOLOGY, 1992, 12 (08) : 3431 - 3438
[8] HAMEL PA, 1992, ONCOGENE, V7, P693
[9] HYPERPHOSPHORYLATION OF THE RETINOBLASTOMA GENE-PRODUCT IS DETERMINED BY DOMAINS OUTSIDE THE SIMIAN VIRUS-40 LARGE-T-ANTIGEN-BINDING REGIONS
HAMEL, PA
COHEN, BL
SORCE, LM
GALLIE, BL
PHILLIPS, RA
[J]. MOLECULAR AND CELLULAR BIOLOGY, 1990, 10 (12) : 6586 - 6595
[10] STRUCTURAL ALTERATIONS AT THE PUTATIVE RETINOBLASTOMA LOCUS IN SOME HUMAN LEUKEMIAS AND PRELEUKEMIA
HANSEN, MF
MORGAN, R
SANDBERG, AA
CAVENEE, WK
[J]. CANCER GENETICS AND CYTOGENETICS, 1990, 49 (01) : 15 - 23

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