PLANT BZIP PROTEINS GATHER AT ACGT ELEMENTS

被引：319

作者：

FOSTER, R ^{[1
]}

IZAWA, T ^{[1
]}

CHUA, NH ^{[1
]}

机构：

[1] ROCKEFELLER UNIV,PLANT MOLEC BIOL LAB,NEW YORK,NY 10021

来源：

FASEB JOURNAL | 1994年 / 8卷 / 02期

关键词：

PROTEIN/DNA INTERACTIONS; TRANSCRIPTIONAL ACTIVATION; DNA BINDING SPECIFICITY; DIMERIZATION; POSTTRANSLATIONAL MODIFICATION; NUCLEAR LOCALIZATION;

D O I：

10.1096/fasebj.8.2.8119490

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：

ACGT cis-acting DNA sequence elements have been identified in a multitude of plant genes regulated by diverse environmental, physiological, and environmental cues. In vivo transient and transgenic plant expression studies have shown that these ACGT elements are necessary for maximal transcriptional activation. Plants possess a conserved family of DNA-binding proteins specific for these DNA sequence motifs. Well-defined in terms of nucleotide sequence required for protein/DNA interactions and transcriptional activation, various ACGT elements have been used as molecular probes to clone sequence-specific DNA binding proteins. All plant DNA-binding proteins specific for ACGT elements belong to the bZIP classification. Most recombinant bZIP proteins can interact with ACGT elements derived from different plant genes, albeit with different affinity. Systematic protein/DNA binding studies have shown that sequences flanking the ACGT core affect bZIP protein binding specificity. These studies have provided the basis for a concise ACGT nomenclature and defined high-affinity A-box, C-box, and G-box elements. Plant bZIP factors can be classified according to their quantitative binding affinities for high-affinity ACGT elements. Potential molecular mechanisms that may control how plant bZIP proteins activate plant gene expression are discussed.

引用

页码：192 / 200

页数：9

共 68 条

[51] INDUCIBLE INVIVO DNA FOOTPRINTS DEFINE SEQUENCES NECESSARY FOR UV-LIGHT ACTIVATION OF THE PARSLEY CHALCONE SYNTHASE GENE [J].

SCHULZE-LEFERT, P ;

DANGL, JL ;

BECKERANDRE, M ;

HAHLBROCK, K ;

SCHULZ, W .

EMBO JOURNAL, 1989, 8 (03) :651-656

[52] OCSBF-1, A MAIZE OCS ENHANCER BINDING-FACTOR - ISOLATION AND EXPRESSION DURING DEVELOPMENT [J].

SINGH, K ;

DENNIS, ES ;

ELLIS, JG ;

LLEWELLYN, DJ ;

TOKUHISA, JG ;

WAHLEITHNER, JA ;

PEACOCK, WJ .

PLANT CELL, 1990, 2 (09) :891-903

[53] A CACGTG MOTIF OF THE ANTIRRHINUM-MAJUS CHALCONE SYNTHASE PROMOTER IS RECOGNIZED BY AN EVOLUTIONARILY CONSERVED NUCLEAR-PROTEIN [J].

STAIGER, D ;

KAULEN, H ;

SCHELL, J .

PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1989, 86 (18) :6930-6934

[54] PURIFICATION OF TOBACCO NUCLEAR PROTEINS BINDING TO A CACGTG MOTIF OF THE CHALCONE SYNTHASE PROMOTER BY DNA AFFINITY-CHROMATOGRAPHY [J].

STAIGER, D ;

BECKER, F ;

SCHELL, J ;

KONCZ, C ;

PALME, K .

EUROPEAN JOURNAL OF BIOCHEMISTRY, 1991, 199 (03) :519-527

[55] IDENTIFICATION OF 3 RESIDUES IN THE BASIC REGIONS OF THE BZIP PROTEINS GCN4, C/EBP AND TAF-1 THAT ARE INVOLVED IN SPECIFIC DNA-BINDING [J].

SUCKOW, M ;

VONWILCKENBERGMANN, B ;

MULLERHILL, B .

EMBO JOURNAL, 1993, 12 (03) :1193-1200

[56] A PROTEIN THAT BINDS TO A CIS-ACTING ELEMENT OF WHEAT HISTONE GENES HAS A LEUCINE ZIPPER MOTIF [J].

TABATA, T ;

TAKASE, H ;

TAKAYAMA, S ;

MIKAMI, K ;

NAKATSUKA, A ;

KAWATA, T ;

NAKAYAMA, T ;

IWABUCHI, M .

SCIENCE, 1989, 245 (4921) :965-967

[57] HBP-1A AND HBP-1B - LEUCINE ZIPPER-TYPE TRANSCRIPTION FACTORS OF WHEAT [J].

TABATA, T ;

NAKAYAMA, T ;

MIKAMI, K ;

IWABUCHI, M .

EMBO JOURNAL, 1991, 10 (06) :1459-1467

[58]

TORRES R, 1992, Current Opinion in Cell Biology, V4, P468, DOI 10.1016/0955-0674(92)90013-3

[59] MUTATIONS OF THE 22-KD AND 27-KD ZEIN PROMOTERS AFFECT TRANSACTIVATION BY THE OPAQUE-2 PROTEIN [J].

UEDA, T ;

WAVERCZAK, W ;

WARD, K ;

SHER, N ;

KETUDAT, M ;

SCHMIDT, RJ ;

MESSING, J .

PLANT CELL, 1992, 4 (06) :701-709

[60]

VANDERKROL AR, 1991, PLANT CELL, V3, P667, DOI 10.1105/tpc.3.7.667

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