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Featured researches published by Indira Rajagopal.


Plant Molecular Biology | 1993

Selection of Arabidopsis cDNAs that partially correct phenotypes of Escherichia coli DNA-damage-sensitive mutants and analysis of two plant cDNAs that appear to express UV-specific dark repari activities

Qishen Pang; John B. Hays; Indira Rajagopal; Timothy S. Schaefer

To resist terrestrial UV radiation, plants employ DNA-damage-repair/toleration (DRT) activities, as well as shielding mechanisms. Little is known about the structure and regulation of plant DRT genes. We isolated DRT cDNAs from Arabidopsis thaliana, by selecting for complementation of Escherichia coli mutants lacking all bacterial defenses against UV-light damage to DNA. These mutants are phenotypically deficient in recombinational and mutagenic toleration (RecA−), excision repair (Uvr−) and photoreactivation toreactivation (Phr−). Among 840 survivors of heavily UV-irradiated (10−7 survival) mutants harboring plasmids derived from an Arabidopsis cDNA library in the vector λYES, we identified four unique plant cDNAs, designated DRT100, DRT101, DRT102, and DRT103. Drt101 and Drt102 activity were specific for UV-light damage, and complemented both UvrB− and UvrC− phenotypes in the dark. Apparent Uvr− correction efficiencies were 1 to 40% for Drt101, and 0.2 to 15% for Drt102, depending on the UV fluence. Drt101 and Drt102 showed no extensive amino-acid homology with any known DNA-repair proteins. Drt100 appeared to correct RecA−, rather than Uvr−, phenotypes. Although the light dependence of Drt103 activity was consistent with its identification as a photoreactivating enzyme, its predicted amino-acid sequence did not resemble known photolyase sequences. The N-terminal coding sequence of Drt101 suggests that it is targeted to chloroplasts, as reported for Drt100. These cDNAs afforded only modest increases in survival during the original selection procedure. The fact that they were readily isolated nevertheless suggests that selections may be made powerful enough to overcome barriers to expression and function in bacteria, at least for cDNAs of reasonable abundance.


DNA Repair | 2005

Stimulation of mutagenesis by proportional deoxyribonucleoside triphosphate accumulation in Escherichia coli.

Linda J. Wheeler; Indira Rajagopal; Christopher K. Mathews


Nucleic Acids Research | 1993

Two cDNAs from the plant Arabidopsis thaliana that partially restore recombination proficiency and DNA-damage resistance to E.coli mutants lacking recombination-intermediate-resolution activities

Qishen Pang; John B. Hays; Indira Rajagopal


Journal of Biological Chemistry | 1995

Roles of vaccinia virus ribonucleotide reductase and glutaredoxin in DNA precursor biosynthesis.

Indira Rajagopal; Byung-Yoon Ahn; Bernard Moss; Christopher K. Mathews


Journal of Biological Chemistry | 2004

Escherichia coli Nucleoside Diphosphate Kinase Interactions with T4 Phage Proteins of Deoxyribonucleotide Synthesis and Possible Regulatory Functions

Rongkun Shen; Michael C. Olcott; JuHyun Kim; Indira Rajagopal; Christopher K. Mathews


Journal of Biological Chemistry | 2005

Adenylate Kinase of Escherichia coli, a Component of the Phage T4 dNTP Synthetase Complex

JuHyun Kim; Rongkun Shen; Michael C. Olcott; Indira Rajagopal; Christopher K. Mathews


Science | 2001

Protein Sequencing in the Post-Genomic Era

Indira Rajagopal; Kevin Ahern


Science | 2000

Genomics Made Easy

Indira Rajagopal


Archive | 2012

Biochemistry Free and Easy

Kevin Ahern; Indira Rajagopal


Science | 1999

All-in-One Sequence Analysis

Indira Rajagopal

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Kevin Ahern

Oregon State University

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John B. Hays

Oregon State University

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JuHyun Kim

Oregon State University

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Qishen Pang

Oregon State University

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Rongkun Shen

Oregon State University

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Bernard Moss

National Institutes of Health

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Byung-Yoon Ahn

National Institutes of Health

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