Single stranded DNA Binding Proteins in Trypanosoma cru*
克鲁锥虫中的单链 DNA 结合蛋白*
基本信息
- 批准号:6530112
- 负责人:
- 金额:$ 4.03万
- 依托单位:
- 依托单位国家:美国
- 项目类别:
- 财政年份:2001
- 资助国家:美国
- 起止时间:2001-08-01 至 2004-07-31
- 项目状态:已结题
- 来源:
- 关键词:DNA binding protein SDS polyacrylamide gel electrophoresis South America Trypanosoma cruzi affinity chromatography confocal scanning microscopy cooperative study fluorescence microscopy gel mobility shift assay gene expression genetic recombination genetic regulation genetic transcription immunofluorescence technique messenger RNA northern blottings nucleic acid repetitive sequence protein degradation protein localization protein purification protein sequence protein structure function protozoal genetics reporter genes southern blotting western blottings
项目摘要
DESCRIPTION (provided by applicant): American trypanosomiasis, or Chagas'
disease is a major public health problem among poor rural populations in Latin
America, where 16-18 million persons suffer from this disease, and 90 million
are at risk. Sharp differences in regulation of gene expression between
trypanosomatids and their mammalian hosts have been described, suggesting this
process as an interesting target for drug design. In these parasites, the
presence of polycistronic transcription means that post-transcriptional
regulation of gene expression is the main step in determining the abundance of
mRNAs. Using nuclear protein fractions from Trypanosoma cruzi epimastigotes,
the group in Uruguay demonstrated the formation of at least three complexes
that specifically recognize two dinucleotide repeated sequences (poly[dT-dG]
and poly[dC-dA]) which are abundant in the vicinity of coding regions of T.
cruzi genes. The specificity and preliminary estimation of equilibrium
constants of these complexes are in good agreement with reported data for gene
regulatory proteins. The goal of this project is to determine whether these
dinucleotide repeats and the proteins that bind to them have a role in
regulation of gene expression, transcription or in selective transcript
processing, degradation or stabilization or recombination. The specific aims of
this FIRCA project are: 1. to characterize the proteins interacting with the
cis target (purification and microsequencing), to determine the fine
subcellular localization of these proteins by immunofluorescence microscopy and
to determine if they show stage specific expression by western analysis. 2. to
characterize the genes encoding these proteins (cloning, sequencing and
analysis by southern blot and chromosomal location as well as northern blot
analysis of their expression). 3. to examine the dinucleotide sequence for
effect on expression of reporter constructs. The location and the minimum
length of the repeat sequence and, if it corresponds, the stage at which
expression is altered [posttranscriptional, translational, etc.] will be
examined. These experimental approaches will lead to an understanding of the
role of these dinucleotide repeated sequences and the function and significance
of the proteins that specifically recognize them providing insights into the
regulation of gene expression in T. cruzi.
描述(由申请人提供):美洲锥虫病或南美锥虫病
项目成果
期刊论文数量(0)
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