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F. Katagiri, E. Lam, N. Chua (1989)
Two tobacco DNA-binding proteins with homology to the nuclear factor CREBNature, 340
R. Fluhr, P. Moses, G. Morelli, G. Coruzzi, N. Chua (1986)
Expression dynamics of the pea rbcS multigene family and organ distribution of the transcriptsThe EMBO Journal, 5
(1985)
Repetitive zincbinding domains in the protein transcription factor MA from Xenopus oocytes
R. Fraley, S. Rogers, R. Horsch, D. Eichholtz, J. Flick, C. Fink, N. Hoffmann, P. Sanders (1985)
The SEV System: A New Disarmed Ti Plasmid Vector System for Plant TransformationBio/Technology, 3
(1989)
Two tobacco DNA-binding proteins have homology to CREB
C. Fromental, M. Kanno, H. Nomiyama, P. Chambon (1988)
Cooperativity and hierarchical levels of functional organization in the SV40 enhancerCell, 54
P. Green, S. Kay, N. Chua (1987)
Sequence‐specific interactions of a pea nuclear factor with light‐responsive elements upstream of the rbcS‐3A gene.The EMBO Journal, 6
J. Miller, A. Mclachlan, A. Klug (1985)
Repetitive zinc‐binding domains in the protein transcription factor IIIA from Xenopus oocytes.The EMBO Journal, 4
C. Kuhlemeier, G. Strittmatter, K. Ward, N. Chua (1989)
The Pea rbcS-3A Promoter Mediates Light Responsiveness but not Organ Specificity.The Plant cell, 1
E. Lam, N. Chua (1989)
ASF-2: a factor that binds to the cauliflower mosaic virus 35S promoter and a conserved GATA motif in Cab promoters.The Plant cell, 1
R. Jefferson, T. Kavanagh, M. Bevan (1987)
GUS fusions: beta‐glucuronidase as a sensitive and versatile gene fusion marker in higher plants.The EMBO Journal, 6
Harinder Singh, J. Lebowitz, A. Baldwin, P. Sharp (1988)
Molecular cloning of an enhancer binding protein:Isolation by screening of an expression library with a recognition site DNACell, 52
R. Fluhr, C. Kuhlemeier, F. Nagy, N. Chua (1986)
Organ-Specific and Light-Induced Expression of Plant GenesScience, 232
(1989)
genes is modulated by phosphorylation
K. Mikami, T. Tabata, T. Kawata, T. Nakayama, M. Iwabuchi (1987)
Nuclear protein(s) binding to the conserved DNA hexameric sequence postulated to regulate transcription of wheat histone genesFEBS Letters, 223
C. Dean, E. Pichersky, P. Dunsmuir (1989)
Structure, evolution and regulation of RbcS genes in higher plants, 40
Expression dynamics of the pea rbcs family and organ distribution of the transcripts
G. Giuliano, E. Pichersky, V. Malik, M. Timko, P. Scolnik, A. Cashmore (1988)
An evolutionarily conserved protein binding sequence upstream of a plant light-regulated gene.Proceedings of the National Academy of Sciences of the United States of America, 85 19
K. Jofuku, J. Okamuro, R. Goldberg (1987)
Interaction of an embryo DNA binding protein with a soybean lectin gene upstream regionNature, 328
C. Kuhlemeier, M. Cuozzo, Pamela Green, Elisabeth Goyvaerts, Kathy Ward, Nam-Hai Chua (1988)
Localization and conditional redundancy of regulatory elements in rbcS-3A, a pea gene encoding the small subunit of ribulose-bisphosphate carboxylase.Proceedings of the National Academy of Sciences of the United States of America, 85 13
Eric Lam, Nam-Hai Chua (1990)
GT-1 binding site confers light responsive expression in transgenic tobacco.Science, 248 4954
P. Benfey, N. Chua (1989)
Regulated Genes in Transgenic PlantsScience, 244
(1987)
GUS fusions : 0 - Glucuronidase as a sensitive and versatile fusion marker in higher plants . EMBO J . 6 , 3901 - 3907
E. Jensen, K. Marcker, J. Schell, F. Bruijn (1988)
Interaction of a nodule specific, trans‐acting factor with distinct DNA elements in the soybean leghaemoglobin Ibc3 5′ upstream regionThe EMBO Journal, 7
F. Nagy, R. Fluhr, C. Kuhlemeier, S. Kay, M. Boutry, P. Green, C. Poulsen, N. Chua (1986)
Cis-Acting Elements for Selective Expression of Two Photosynthetic Genes in Transgenic PlantsPhilosophical Transactions of the Royal Society B, 314
A. Maxam, W. Gilbert (1980)
Sequencing end-labeled DNA with base-specific chemical cleavages.Methods in enzymology, 65 1
K. Struhl (1989)
Helix-turn-helix, zinc-finger, and leucine-zipper motifs for eukaryotic transcriptional regulatory proteins.Trends in biochemical sciences, 14 4
P. Green, Mun‐Heng Yong, M. Cuozzo, Y. Kano-Murakami, P. Silverstein, N. Chua (1988)
Binding site requirements for pea nuclear protein factor GT‐1 correlate with sequences required for light‐dependent transcriptional activation of the rbcS‐3A gene.The EMBO Journal, 7
(1987)
GUS fusions: 0-Glucuronidase as a sensitive and versatile fusion marker in higher plants
P. Benfey, L. Ren, N. Chua (1989)
The CaMV 35S enhancer contains at least two domains which can confer different developmental and tissue‐specific expression patternsThe EMBO Journal, 8
M. Bustos, M. Guiltinan, J. Jordano, Dilara Begum, F. Kalkan, Timothy Hall (1989)
Regulation of beta-glucuronidase expression in transgenic tobacco plants by an A/T-rich, cis-acting sequence found upstream of a French bean beta-phaseolin gene.The Plant cell, 1
E. Lam, P. Benfey, P. Gilmartin, R. Fang, N. Chua (1989)
Site-specific mutations alter in vitro factor binding and change promoter expression pattern in transgenic plants.Proceedings of the National Academy of Sciences of the United States of America, 86 20
Regulation of Psglucuronidase expression in transgenic tobacco plants by an A / T - rich , cis - acting sequence found upstream of a French bean P - phaseolin gene
Neeraj Datta, A. Cashmore (1989)
Binding of a pea nuclear protein to promoters of certain photoregulated genes is modulated by phosphorylation.The Plant cell, 1
Abstract We have used DNase I footprinting to characterize nuclear factors that bind to the light-responsive promoter of pea rbcS-3A, one member of the gene family encoding the small subunit of ribulose-1,5-bisphosphate carboxylase. A sequence-specific binding activity, designated 3AF1, binds to an AT-rich sequence present at the -45 region of the rbcS-3A promoter. A tetramer of the 3AF1 binding site, designated as Box VI, can form multiple complexes with tobacco leaf and root nuclear extracts. Mutations of 3 base pairs in Box VI severely reduce DNA-protein complex formation in vitro. The wild-type Box VI tetramer, but not the mutant tetramer, is active in transgenic tobacco plants when placed upstream of the cauliflower mosaic virus 35S promoter truncated at -90. These results correlate binding of 3AF1 to the in vivo function of Box VI. The Box VI tetramer/35S chimeric construct confers expression in diverse cell types and organs and its activity is not dependent on light. By using the Box VI tetramer as a probe to screen a cDNA expression library, we have obtained a putative cDNA clone for the 3AF1 DNA-binding activity. Lysogen extracts of Escherichia coli expressing the cDNA clone give sequence-specific complexes with Box VI. The deduced amino acid sequence of the protein encoded by the cDNA contains two stretches of about 100 residues that are 80% homologous. Moreover, in each of the two repeats, there is an arrangement of histidines and cysteines, which may be related to the two known types of zinc-finger motifs found in many DNA-binding proteins. Consistent with the expectation that metal coordination plays an important role in DNA binding by this protein, we found that 1,10-phenanthroline can abolish the formation of DNA-protein complexes. Interestingly, we found that the same treatment did not abolish the DNA binding activity of 3AF1 in crude nuclear extracts of tobacco. These data indicate that the nuclear 3AF1 activity is likely due to multiple DNA-binding proteins all interacting with Box VI in vitro. RNA gel blot analysis shows that multiple transcripts homologous to this cDNA clone are expressed in different tobacco organs. This content is only available as a PDF. © 1990 by American Society of Plant Biologists This article is published and distributed under the terms of the Oxford University Press, Standard Journals Publication Model (https://academic.oup.com/journals/pages/open_access/funder_policies/chorus/standard_publication_model)
The Plant Cell – Oxford University Press
Published: Sep 1, 1990
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