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Tools for target identification and
validation
By sreeremya.s
Asst professor,sree narayana guru
college,cbe
• Microarrays
• Target identification seeks to identify new targets, normally
• proteins (or DNA/RNA), whose modulation might
• inhibit or reverse disease progression. Current technologies
• enable researchers to attempt to correlate changes in
• gene (genomics) and protein (proteomics) expression
• with human disease, in the hope of finding new targets.
• Microarrays are a well-utilized tool in both academic and
• industrial research laboratories. They can be used to
• assess gene and protein expression (via nucleic acid or
• protein microarrays) to identify novel targets, and can also
• be used to validate the found targets at the tissue or cell
• scale (via tissue or cell microarrays
• Nucleic acid microarrays
• Today, nucleic-acid microarrays, which primarily use
• short oligonucleotides (15–25 nt), long oligonucleotides
• (50–120 nt) and PCR-amplified cDNAs (100–3000 base
• pairs) as array elements, are overwhelmingly dominant
• because of the relatively easy synthesis and the chemical
• robustness of DNA [8]. Data generated from genome
• sequencing projects in several organisms has provided the
• opportunity to build comprehensive maps of transcriptional
• regulation. Array-based gene expression analysis
• (immobilized DNA probes hybridizing to RNA or cDNA
• targets) has enabled parallel monitoring of cellular transcription
• at the level of the genome.
• Protein microarrays
• Because most drug targets are proteins, protein and
peptide
• microarrays are set to have an important impact on
• drug discovery. Protein arrays, an emerging yet very
• promising technology, are now being used to examine
• enzyme–substrate, DNA–protein and protein–protein
• interactions [10]. By profiling the differential expression
• of proteins using antibody arrays and correlating the
• changes to a disease phenotype, putative targets (and
• biomarkers) to a particular disease can be identified
• Tissue and cell microarrays
• Almost all published tissue microarray studies have been
• related to the analysis of tumors [13,15]. An alternative to
• the use of whole-tissue specimens is the use of live cell
• microarrays, which can be used to identify potential drug
• targets by functionally characterizing large numbers of
• gene products in cell-based assays. In one example [13],
• a tissue microarray was constructed using 210 human
• HCCs and corresponding normal liver, and followed by
• immunohistochemical analysis to test the clinical value of
• the proteins that have been identified.
• Besides being used as an essential step in analyzing highthroughput
• experiments such as DNA microarrays, bioinformatics
• can contribute to the processes of target
• identification and validation by providing functional
• information of target candidates and positioning information
• on the biological networks. Numerous public biological
• databases are warehousing and providing a great
• amount of functional information for genes or proteins,
• and many useful bioinformatics tools are continuously
• developed. Enriched information and the bioinformatics
• tools have enabled in silico cloning of target candidates.
• SNAIL3, a potent target of pharmacogenomics in the
• field of oncology and regenerative medicine, is an example
• for in silico isolation by proper combination of available
• bioinformatics tools and information
• Antisense oligonucleotides
• Complementary to a portion of a target mRNA
molecule,
• oligonucleotides are the original type of molecule used
for
• blocking protein synthesis of the target mRNA, and
thus
• achieving the knockdown of the target gene [20]. One
• example is the identification of COX17 as a therapeutic
• target for non-small cell lung cancer (NSCLC) [21].
• Following the observation of overexpression of the
• COX17 transcript on a cDNA microarray, increased
• expression of COX17 in all of eight primary NSCLCs
• and in 11 of 15 NSCLC cell lines examined was documented
• using semiquantitative reverse transcription-
• PCR, by comparison with normal lung tissue. Treatment
• of NSCLC cells with antisense S-oligonucleotides or
• vector-based small interfering RNAs of COX17 suppressed
• expression of COX17 and also suppressed growth
• of the cancer cells. Combined with other data, this suggests
• that selective suppression of COX17 expression
• could form a promising new strategy for treating lung
• cancers.
Tools for target identification and validation using microarrays
Tools for target identification and validation using microarrays
Tools for target identification and validation using microarrays
Tools for target identification and validation using microarrays
Tools for target identification and validation using microarrays

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Tools for target identification and validation using microarrays

  • 1. Tools for target identification and validation By sreeremya.s Asst professor,sree narayana guru college,cbe
  • 2. • Microarrays • Target identification seeks to identify new targets, normally • proteins (or DNA/RNA), whose modulation might • inhibit or reverse disease progression. Current technologies • enable researchers to attempt to correlate changes in • gene (genomics) and protein (proteomics) expression • with human disease, in the hope of finding new targets. • Microarrays are a well-utilized tool in both academic and • industrial research laboratories. They can be used to • assess gene and protein expression (via nucleic acid or • protein microarrays) to identify novel targets, and can also • be used to validate the found targets at the tissue or cell • scale (via tissue or cell microarrays
  • 3. • Nucleic acid microarrays • Today, nucleic-acid microarrays, which primarily use • short oligonucleotides (15–25 nt), long oligonucleotides • (50–120 nt) and PCR-amplified cDNAs (100–3000 base • pairs) as array elements, are overwhelmingly dominant • because of the relatively easy synthesis and the chemical • robustness of DNA [8]. Data generated from genome • sequencing projects in several organisms has provided the • opportunity to build comprehensive maps of transcriptional • regulation. Array-based gene expression analysis • (immobilized DNA probes hybridizing to RNA or cDNA • targets) has enabled parallel monitoring of cellular transcription • at the level of the genome.
  • 4. • Protein microarrays • Because most drug targets are proteins, protein and peptide • microarrays are set to have an important impact on • drug discovery. Protein arrays, an emerging yet very • promising technology, are now being used to examine • enzyme–substrate, DNA–protein and protein–protein • interactions [10]. By profiling the differential expression • of proteins using antibody arrays and correlating the • changes to a disease phenotype, putative targets (and • biomarkers) to a particular disease can be identified
  • 5. • Tissue and cell microarrays • Almost all published tissue microarray studies have been • related to the analysis of tumors [13,15]. An alternative to • the use of whole-tissue specimens is the use of live cell • microarrays, which can be used to identify potential drug • targets by functionally characterizing large numbers of • gene products in cell-based assays. In one example [13], • a tissue microarray was constructed using 210 human • HCCs and corresponding normal liver, and followed by • immunohistochemical analysis to test the clinical value of • the proteins that have been identified.
  • 6. • Besides being used as an essential step in analyzing highthroughput • experiments such as DNA microarrays, bioinformatics • can contribute to the processes of target • identification and validation by providing functional • information of target candidates and positioning information • on the biological networks. Numerous public biological • databases are warehousing and providing a great • amount of functional information for genes or proteins, • and many useful bioinformatics tools are continuously • developed. Enriched information and the bioinformatics • tools have enabled in silico cloning of target candidates. • SNAIL3, a potent target of pharmacogenomics in the • field of oncology and regenerative medicine, is an example • for in silico isolation by proper combination of available • bioinformatics tools and information
  • 7. • Antisense oligonucleotides • Complementary to a portion of a target mRNA molecule, • oligonucleotides are the original type of molecule used for • blocking protein synthesis of the target mRNA, and thus • achieving the knockdown of the target gene [20]. One • example is the identification of COX17 as a therapeutic • target for non-small cell lung cancer (NSCLC) [21].
  • 8. • Following the observation of overexpression of the • COX17 transcript on a cDNA microarray, increased • expression of COX17 in all of eight primary NSCLCs • and in 11 of 15 NSCLC cell lines examined was documented • using semiquantitative reverse transcription- • PCR, by comparison with normal lung tissue. Treatment • of NSCLC cells with antisense S-oligonucleotides or • vector-based small interfering RNAs of COX17 suppressed • expression of COX17 and also suppressed growth • of the cancer cells. Combined with other data, this suggests • that selective suppression of COX17 expression • could form a promising new strategy for treating lung • cancers.