DOCSLIB.ORG

Anti-TCF7L1 Monoclonal Antibody, Clone FQS3142 (DCABH-2698) This Product Is for Research Use Only and Is Not Intended for Diagnostic Use

Total Page:16

File Type:pdf, Size:1020Kb

Download full-text PDF Read full-text
Anti-TCF7L1 Monoclonal Antibody, Clone FQS3142 (DCABH-2698) This Product Is for Research Use Only and Is Not Intended for Diagnostic Use Anti-TCF7L1 monoclonal antibody, clone FQS3142 (DCABH-2698) This product is for research use only and is not intended for diagnostic use. PRODUCT INFORMATION Product Overview Rabbit monoclonal to TCF7L1 Antigen Description Participates in the Wnt signaling pathway. Binds to DNA and acts as a repressor in the absence of CTNNB1, and as an activator in its presence. Necessary for the terminal differentiation of epidermal cells, the formation of keratohyalin granules and the development of the barrier function of the epidermis (By similarity). Down-regulates NQO1, leading to increased mitomycin c resistance. Immunogen Synthetic peptide corresponding to residues in Human TCF7L1 (UniProt Q9HCS4). Isotype IgG Source/Host Rabbit Species Reactivity Human Clone FQS3142 Purity Tissue culture supernatant Conjugate Unconjugated Applications WB, Flow Cyt Positive Control A431 and Human fetal small intestine lysates Format Liquid Size 100 μl Buffer pH: 7.40; Preservative: 0.01% Sodium azide; Constituents: 50% Glycerol, 0.05% BSA Preservative 0.01% Sodium Azide Storage Store at -20°C. Stable for 12 months at -20°C GENE INFORMATION 45-1 Ramsey Road, Shirley, NY 11967, USA Email: [email protected] Tel: 1-631-624-4882 Fax: 1-631-938-8221 1 © Creative Diagnostics All Rights Reserved Gene Name TCF7L1 transcription factor 7-like 1 (T-cell specific, HMG-box) [ Homo sapiens ] Official Symbol TCF7L1 Synonyms TCF7L1; transcription factor 7-like 1 (T-cell specific, HMG-box); TCF3; transcription factor 7-like 1; HMG box transcription factor 3; TCF-3; Entrez Gene ID 83439 Protein Refseq NP_112573 UniProt ID Q9HCS4 Chromosome Location 2p11.2 Pathway Acute myeloid leukemia, organism-specific biosystem; Acute myeloid leukemia, conserved biosystem; Adherens junction, organism-specific biosystem; Adherens junction, conserved biosystem; Arrhythmogenic right ventricular cardiomyopathy (ARVC), organism-specific biosystem; Arrhythmogenic right ventricular cardiomyopathy (ARVC), conserved biosystem; Basal cell carcinoma, organism-specific biosystem; Function DNA binding; beta-catenin binding; chromatin binding; sequence-specific DNA binding; sequence-specific DNA binding transcription factor activity; sequence-specific DNA binding transcription factor activity; transcription regulatory region DNA binding; 45-1 Ramsey Road, Shirley, NY 11967, USA Email: [email protected] Tel: 1-631-624-4882 Fax: 1-631-938-8221 2 © Creative Diagnostics All Rights Reserved.
Load more

Recommended publications
  • Genome-Wide Linkage and Admixture Mapping of Type 2 Diabetes In
    ORIGINAL ARTICLE Genome-Wide Linkage and Admixture Mapping of Type 2 Diabetes in African American Families From the American Diabetes Association GENNID (Genetics of NIDDM) Study Cohort Steven C. Elbein,1,2 Swapan K. Das,1,2 D. Michael Hallman,3 Craig L. Hanis,3 and Sandra J. Hasstedt4 OBJECTIVE—We used a single nucleotide polymorphism (SNP) map in a large cohort of 580 African American families to identify regions linked to type 2 diabetes, age of type 2 diabetes ype 2 diabetes is marked by a clear genetic diagnosis, and BMI. propensity, a high concordance in identical twins, tendencies for both diabetes and age of RESEARCH DESIGN AND METHODS—After removing outli- onset to be familial (1), and marked differences ers and problematic samples, we conducted linkage analysis T in prevalence among ethnic groups (2). Despite consider- using 5,914 SNPs in 1,344 individuals from 530 families. Linkage analysis was conducted using variance components for type 2 able evidence for a genetic predisposition, unraveling the diabetes, age of type 2 diabetes diagnosis, and BMI and nonpara- genetic etiology has been daunting, with few confirmed metric linkage analyses. Ordered subset analyses were con- genes identified from genome-wide linkage scans. Recent ducted ranking on age of type 2 diabetes diagnosis, BMI, waist successes with genome-wide association scans (3) have circumference, waist-to-hip ratio, and amount of European ad- greatly increased the number of confirmed genetic loci, mixture. Admixture mapping was conducted using 4,486 markers but these successes have been limited primarily to Cauca- not in linkage disequilibrium.
    [Show full text]
  • Wnt Suppressor and Stem Cell Regulator TCF7L1 Is a Sensitive
    Experimental and Molecular Pathology 110 (2019) 104293 Contents lists available at ScienceDirect Experimental and Molecular Pathology journal homepage: www.elsevier.com/locate/yexmp Wnt suppressor and stem cell regulator TCF7L1 is a sensitive immunohistochemical marker to differentiate testicular seminoma from T non-seminomatous germ cell tumor ⁎ Lihong Bua, Qi Yangb, Loralee McMahonb, Guang-Qian Xiaob,c, Faqian Lia,b,d, a Department of Laboratory Medicine and Pathology, University of Minnesota, 420 Delaware Street SE, Minneapolis, MN 55455, United States of America b Department of Pathology and Laboratory Medicine, University of Rochester Medical Center, 601 Elmwood Avenue, Rochester, NY 14642, United States of America c Department of Pathology, Keck School of Medicine, University of Southern California, 2011 Zonal Avenue, Los Angeles, CA 90089, United States of America d Lillehei Heart Institute and Masonic Cancer Center, University of Minnesota, Minneapolis, MN 55455, United States of America ARTICLE INFO ABSTRACT Keywords: The accurate classification and proper identification of testicular germ cell tumors is imperative for treatment Wnt selection and clinical prognosis. Although such distinction can often be achieved by microscopic morphology TCF7L1 alone, ancillary tests may at times be needed. T-cell factor 7 L1 (TCF7L1, also known as TCF3), a component of Germ cell tumor the Wnt signaling pathway, plays important roles in embryonic stem cell self-renewal and lineage specification. Seminoma Here we examined the immunohistochemical expression and diagnostic utility of TCF7L1 in testicular germ cell Non-seminomatous tumors. Fifty cases of testicular germ cell tumors were collected, including 23 seminomas, 6 embryonal carci- Mixed germ cell tumor Embryonal carcinoma nomas, 1 teratoma, 1 choriocarcinoma, and 19 mixed germ cell tumors.
    [Show full text]
  • Endogenous Bioid Elucidates TCF7L1 Interactome Modulation Upon GSK-3 Inhibition in Mouse Escs
    bioRxiv preprint doi: https://doi.org/10.1101/431023; this version posted October 1, 2018. The copyright holder for this preprint (which was not certified by peer review) is the author/funder. All rights reserved. No reuse allowed without permission. Endogenous BioID elucidates TCF7L1 interactome modulation upon GSK-3 inhibition in mouse ESCs Steven Moreira1, Caleb Seo1, Victor Gordon1, Sansi Xing1, Ruilin Wu1, Enio Polena1, Vincent Fung1, Deborah Ng2,3, Cassandra J Wong4,5, Brett Larsen4,5, Brian Raught2,3, Anne-Claude Gingras4,5, Yu Lu1, and Bradley W. Doble1. 1Department of Biochemistry and Biomedical Sciences, Stem Cell and Cancer Research Institute, McMaster University, Hamilton, ON L8N 3Z5, Canada 2Princess Margaret Cancer Centre, University Health Network, 101 College Street, Toronto, ON M5G 1L7, Canada 3Department of Medical Biophysics, University of Toronto, Toronto, ON M5G 1L7, Canada 4Lunenfeld-Tanenbaum Research Institute, Mount Sinai Hospital, 600 University Avenue, Toronto, ON M5G 1X5, Canada 5Department of Molecular Genetics, University of Toronto, Toronto, ON M5S 1A8, Canada Modulation of Wnt target gene expression via the TCF/LEFs interactions with the T-Cell Factor/Lymphoid Enhancer Fac- remains poorly understood. We employ proximity-based bi- tor (TCF/LEF) family of transcription factors (3). otin labeling (BioID) to examine GSK-3 inhibitor effects on In mouse embryonic stem cells (mESCs) all four TCF/LEF the TCF7L1 interactome in mouse ESCs. We generated ESC family members, TCF7, TCF7L1, TCF7L2, and LEF1 are ex- lines with biotin ligase BirA* fused to TCF7L1 by knocking it into the endogenous TCF7L1 locus or by inserting a dox- pressed at detectable protein levels (4, 5), although TCF7L1 inducible BirA*-TCF7L1 transgene into the Rosa26 locus.
    [Show full text]
  • A B-Catenin-Driven Switch in TCF/LEF Transcription Factor Binding To
    RESEARCH ARTICLE A b-catenin-driven switch in TCF/LEF transcription factor binding to DNA target sites promotes commitment of mammalian nephron progenitor cells Qiuyu Guo1, Albert Kim1, Bin Li2, Andrew Ransick1, Helena Bugacov1, Xi Chen1, Nils Lindstro¨ m1, Aaron Brown3, Leif Oxburgh2, Bing Ren4, Andrew P McMahon1* 1Department of Stem Cell Biology and Regenerative Medicine, Eli and Edythe Broad-CIRM Center for Regenerative Medicine and Stem Cell Research, Keck School of Medicine of the University of Southern California, Los Angeles, United States; 2The Rogosin Institute, New York, United States; 3Center for Molecular Medicine, Maine Medical Center Research Institute, Scarborough, United States; 4Ludwig Institute for Cancer Research, Department of Cellular and Molecular Medicine, Institute of Genomic Medicine, Moores Cancer Center, University of California San Diego, San Diego, United States Abstract The canonical Wnt pathway transcriptional co-activator b-catenin regulates self-renewal and differentiation of mammalian nephron progenitor cells (NPCs). We modulated b-catenin levels in NPC cultures using the GSK3 inhibitor CHIR99021 (CHIR) to examine opposing developmental actions of b-catenin. Low CHIR-mediated maintenance and expansion of NPCs are independent of direct engagement of TCF/LEF/b-catenin transcriptional complexes at low CHIR-dependent cell- cycle targets. In contrast, in high CHIR, TCF7/LEF1/b-catenin complexes replaced TCF7L1/TCF7L2 binding on enhancers of differentiation-promoting target genes. Chromosome confirmation studies
    [Show full text]
  • Multiomics Data Integration Unveils Core Transcriptional Regulatory Networks Governing Cell-Type Identity ✉ Sascha Jung1 and Antonio Del Sol 1,2,3,4
    www.nature.com/npjsba BRIEF COMMUNICATION OPEN Multiomics data integration unveils core transcriptional regulatory networks governing cell-type identity ✉ Sascha Jung1 and Antonio del Sol 1,2,3,4 A plethora of computational approaches have been proposed for reconstructing gene regulatory networks (GRNs) from gene expression data. However, gene regulatory processes are often too complex to predict from the transcriptome alone. Here, we present a computational method, Moni, that systematically integrates epigenetics, transcriptomics, and protein–protein interactions to reconstruct GRNs among core transcription factors and their co-factors governing cell identity. We applied Moni to 57 datasets of human cell types and lines and demonstrate that it can accurately infer GRNs, thereby outperforming state-of-the-art methods. npj Systems Biology and Applications (2020) 6:26 ; https://doi.org/10.1038/s41540-020-00148-4 INTRODUCTION lines assembled from ArchS4 (ref. 15). Based on a previous study Cellular phenotypes are characterized by stable gene expression demonstrating that the TFs with the highest phenotypic specificity 16 profiles maintained by a set of transcription factors (TFs) that are most likely to be essential determinants of cell identity , the jointly determine cell identity. Together with other co-factors, 10 TFs with the highest phenotypic specificity are selected as core 1234567890():,; these identity TFs form a regulatory core network, which is shaped TFs. In addition, potential co-factors are detected, i.e., TFs that are by the epigenetic landscape1–3. In particular, the epigenetic significantly more specific to the phenotype than their expected landscape, defined by epigenetic modifications, chromatin acces- median specificity. Secondly, active promoters and enhancers of sibility, and chromatin conformation, determines phenotype- core TFs and co-factors are identified.
    [Show full text]
  • Working Party of National Coordinators of the Test Guidelines Programme
    Organisation for Economic Co-operation and Development ENV/CBC/TG(2021)31 For Official Use English - Or. English 7 May 2021 ENVIRONMENT DIRECTORATE CHEMICALS AND BIOTECHNOLOGY COMMITTEE Working Party of National Coordinators of the Test Guidelines Programme Adverse Outcome Pathway 220 on Cyp2E1 Activation Leading to Liver Cancer Nathalie Delrue, Administrator [email protected] JT03476102 OFDE This document, as well as any data and map included herein, are without prejudice to the status of or sovereignty over any territory, to the delimitation of international frontiers and boundaries and to the name of any territory, city or area. 2 ENV/CBC/TG(2021)31 Foreword This Adverse Outcome Pathway (AOP) on Cyp2E1 Activation Leading to Liver Cancer, has been developed under the auspices of the OECD AOP Development Programme, overseen by the Extended Advisory Group on Molecular Screening and Toxicogenomics (EAGMST), which is an advisory group under the Working Party of the National Coordinators of the Test Guidelines Programme (WNT). The AOP has been reviewed internally by the EAGMST, externally by experts nominated by the WNT, and has been endorsed by the WNT and the Working Party on Hazard Assessment (WPHA) on XXX. Through endorsement of this AOP, the WNT and the WPHA express confidence in the scientific review process that the AOP has undergone and accept the recommendation of the EAGMST that the AOP be disseminated publicly. Endorsement does not necessarily indicate that the AOP is now considered a tool for direct regulatory application. The OECD's Chemicals and Biotechnology Committee agreed to declassification of this AOP on XXX.
    [Show full text]
  • Dna Methylation Changes in Whole Blood and Cd16+ Neutrophils In
    DNA METHYLATION CHANGES IN WHOLE BLOOD AND CD16+ NEUTROPHILS IN RESPONSE TO CHRONIC FOLIC ACID SUPPLEMENTATION IN WOMEN OF CHILD-BEARING AGE by DEANNA SHADE (Under the Direction of Dorothy B. Hausman) ABSTRACT The aim of this study was to determine if DNA methylation in a single leukocyte type would respond differently than whole blood (WB) in response to folic acid (FA) supplementation. This study was performed in normal weight women (18-35 y; n = 12), with blood samples taken before and after 8 weeks of supplementation with 800 μg/day of FA. DNA methylation patterns from WB and CD16+ neutrophils (CD16) were measured across 485,000 CpG sites. We identified 7839 and 8317 sites that changed (P<0.05) in WB and CD16, respectively with decreases in methylation in 77.2% (WB) and 65.6% (CD16) of these sites. These results suggest that the genome-wide DNA methylation response to FA supplementation is different in WB and CD16. Future studies should measure DNA methylation response to FA supplementation in other leukocyte types to determine if a single cell type could act as a more reliable epigenetic reporter than WB. INDEX WORDS: Women of child-bearing age, Folate, Folic acid, One-carbon metabolism, DNA methylation, Genome-wide, Whole blood, CD16+ neutrophil DNA METHYLATION CHANGES IN WHOLE BLOOD AND CD16+ NEUTROPHILS IN RESPONSE TO CHRONIC FOLIC ACID SUPPLEMENTATION IN WOMEN OF CHILD-BEARING AGE By DEANNA SHADE B.S., The University of Florida, 2012 A Thesis Submitted to the Graduate Faculty of The University of Georgia in Partial Fulfillment
    [Show full text]
  • Repressor Transcription Factor 7-Like 1 Promotes Adipogenic Competency in Precursor Cells
    Repressor transcription factor 7-like 1 promotes adipogenic competency in precursor cells Ana G. Cristanchoa, Michael Schuppa, Martina I. Lefterovaa, Shengya Caoa, Daniel M. Cohenb, Christopher S. Chenb, David J. Stegera, and Mitchell A. Lazara,1 aDivision of Endocrinology, Diabetes, and Metabolism, Departments of Medicine and Genetics and Institute for Diabetes, Obesity, and Metabolism, Perelman School of Medicine at the University of Pennsylvania; and bDepartment of Bioengineering, University of Pennsylvania, Philadelphia, PA 19104 Edited by Bruce M. Spiegelman, Dana-Farber Cancer Institute/Harvard Medical School, Boston, MA, and approved August 15, 2011 (received for review June 10, 2011) The identification of factors that define adipocyte precursor poten- found that cell shape regulation is essential for determining line- tial has important implications for obesity. Preadipocytes are age decisions in mesenchymal stem cells (MSCs) (22, 24, 25). In- fibroblastoid cells committed to becoming round lipid-laden adipo- terestingly, many of the genes repressed early after the addition of cytes. In vitro, this differentiation process is facilitated by conflu- adipogenic stimuli to confluent preadipocytes are regulators of cell ency, followed by adipogenic stimuli. During adipogenesis, a large structure (26–28). The repressed cell structure genes are not γ α number of cytostructural genes are repressed before adipocyte enriched as genomic targets for PPAR or C/EBP (8, 9), sug- gene induction. Here we report that the transcriptional repressor gesting a role for an as-yet unknown transcriptional repressor in transcription factor 7-like 1 (TCF7L1) binds and directly regulates the regulation of cell shape during adipocyte differentiation. expression of cell structure genes. Depletion of TCF7L1 inhibits Transcription factor 7-like 1 (TCF7L1, formerly known as differentiation, because TCF7L1 indirectly induces the adipogenic TCF3) is an intriguing candidate for such a repressor.
    [Show full text]
  • Alternative Splicing Regulates Mouse Embryonic Stem Cell Pluripotency and Differentiation
    Alternative splicing regulates mouse embryonic stem cell pluripotency and differentiation Nathan Salomonisa,b,1, Christopher R. Schlievea, Laura Pereirac, Christine Wahlquistd, Alexandre Colasd, Alexander C. Zambone, Karen Vranizanf,2, Matthew J. Spindlera,b, Alexander R. Picoa, Melissa S. Clineg, Tyson A. Clarkg, Alan Williamsg, John E. Blumeg, Eva Samala, Mark Mercolad, Bradley J. Merrillc, and Bruce R. Conklina,b,h,1 aGladstone Institute of Cardiovascular Disease, San Francisco, CA 94158; bPharmaceutical Sciences and Pharmacogenomics Graduate Program, University of California, San Francisco, CA 94143; cDepartment of Biochemistry and Molecular Genetics, University of Illinois, Chicago, IL 60607; dSanford-Burnham Institute for Medical Research, La Jolla, CA 92037; eDepartment of Pharmacology, University of California, La Jolla, CA 92093; fFunctional Genomics Laboratory, University of California, Berkeley, CA 94720; gAffymetrix, Inc., Santa Clara, CA 95051; and hDepartments of Medicine and Cellular and Molecular Pharmacology, University of California, San Francisco, CA 94143 Edited by Elaine Fuchs, The Rockefeller University, New York, NY, and approved April 27, 2010 (received for review October 27, 2009) Two major goals of regenerative medicine are to reproducibly APS appear to increase transcript diversity in ES cells and thus transform adult somatic cells into a pluripotent state and to con- are likely to affect differentiation to distinct tissue lineages (10– trol their differentiation into specific cell fates. Progress toward 13). A better understanding of how AS regulates protein di- these goals would be greatly helped by obtaining a complete pic- versity and translational repression during ES cell differentiation ture of the RNA isoforms produced by these cells due to alterna- may provide critical insights into this process.
    [Show full text]
  • Nuclear Regulation of Wnt/-Catenin Signaling
    G C A T T A C G G C A T genes Review Nuclear Regulation of Wnt/β-Catenin Signaling: It’s a Complex Situation Christin C. Anthony 1 , David J. Robbins 2, Yashi Ahmed 3 and Ethan Lee 1,4,* 1 Department of Cell & Developmental Biology, Vanderbilt University, Nashville, TN 37232, USA; [email protected] 2 Molecular Oncology Program, Division of Surgical Oncology, Dewitt Daughtry Family Department of Surgery, and Sylvester Comprehensive Cancer Center, Miller School of Medicine, University of Miami, Miami, FL 33136, USA; [email protected] 3 Department of Molecular and Systems Biology and the Norris Cotton Cancer Center, Geisel School of Medicine at Dartmouth College, Hanover, NH 03755, USA; [email protected] 4 Vanderbilt Ingram Cancer Center, Vanderbilt University Medical Center, Nashville, TN 37232, USA * Correspondence: [email protected] Received: 14 July 2020; Accepted: 31 July 2020; Published: 4 August 2020 Abstract: Wnt signaling is an evolutionarily conserved metazoan cell communication pathway required for proper animal development. Of the myriad of signaling events that have been ascribed to cellular activation by Wnt ligands, the canonical Wnt/β-catenin pathway has been the most studied and best understood. Misregulation of Wnt/β-catenin signaling has been implicated in developmental defects in the embryo and major diseases in the adult. Despite the latter, no drugs that inhibit the Wnt/β-catenin pathway have been approved by the FDA. In this review, we explore the least understood step in the Wnt/β-catenin pathway—nuclear regulation of Wnt target gene transcription. We initially describe our current understanding of the importation of β-catenin into the nucleus.
    [Show full text]
  • TCF7L1 (NM 031283) Human Tagged ORF Clone Product Data
    OriGene Technologies, Inc. 9620 Medical Center Drive, Ste 200 Rockville, MD 20850, US Phone: +1-888-267-4436 [email protected] EU: [email protected] CN: [email protected] Product datasheet for RC208913 TCF7L1 (NM_031283) Human Tagged ORF Clone Product data: Product Type: Expression Plasmids Product Name: TCF7L1 (NM_031283) Human Tagged ORF Clone Tag: Myc-DDK Symbol: TCF7L1 Synonyms: TCF-3; TCF3 Vector: pCMV6-Entry (PS100001) E. coli Selection: Kanamycin (25 ug/mL) Cell Selection: Neomycin This product is to be used for laboratory only. Not for diagnostic or therapeutic use. View online » ©2021 OriGene Technologies, Inc., 9620 Medical Center Drive, Ste 200, Rockville, MD 20850, US 1 / 4 TCF7L1 (NM_031283) Human Tagged ORF Clone – RC208913 ORF Nucleotide >RC208913 representing NM_031283 Sequence: Red=Cloning site Blue=ORF Green=Tags(s) TTTTGTAATACGACTCACTATAGGGCGGCCGGGAATTCGTCGACTGGATCCGGTACCGAGGAGATCTGCC GCCGCGATCGCC ATGCCCCAGCTCGGCGGCGGGGGCGGCGGCGGCGGCGGCGGCAGCGGGGGAGGCGGCGGCTCCAGCGCCG GGGCGGCCGGCGGAGGGGACGACCTCGGGGCGAACGACGAGCTGATCCCCTTCCAGGACGAGGGGGGCGA GGAGCAGGAGCCGAGCAGCGATAGCGCCTCGGCGCAGCGGGACCTAGACGAGGTCAAGTCGTCCCTGGTC AACGAGTCGGAGAACCAGAGCAGCAGCTCGGACTCGGAGGCGGAGAGGCGCCCGCAGCCCGTCCGGGACA CTTTCCAGAAGCCGCGGGACTATTTCGCCGAAGTGAGAAGGCCTCAGGACAGCGCGTTCTTTAAAGGACC CCCGTACCCTGGGTACCCCTTCCTGATGATCCCGGACCTGAGCAGCCCGTACCTCTCCAACGGACCCCTG TCTCCCGGAGGAGCGCGCACCTACCTGCAGATGAAATGGCCCCTCCTCGATGTCCCCTCCAGCGCCACAG TCAAGGACACGAGGTCACCATCTCCAGCACACTTGTCTAATAAAGTTCCTGTCGTTCAGCACCCGCATCA CATGCATCCGCTGACTCCCCTCATCACCTACAGCAATGACCACTTCTCCCCCGGCTCCCCTCCCACCCAC
    [Show full text]
  • Snps) in Human T- Cell Acute Lymphocytic Leukemia Protein 1 (TAL1) Gene/ Comprehensive Study
    bioRxiv preprint doi: https://doi.org/10.1101/447540; this version posted October 19, 2018. The copyright holder for this preprint (which was not certified by peer review) is the author/funder. All rights reserved. No reuse allowed without permission. Computational Analysis of Single Nucleotide polymorphisms (SNPs) in Human T- Cell Acute Lymphocytic Leukemia Protein 1 (TAL1) Gene/ Comprehensive Study Shaza W. Shantier1*, Hashim E. Elmansi2, Mihad E. Elnnewery3, Hind K. Osman2, Isam-Aldin A. Alhassan2, Fatima A. Abdelrhman2,Ahmed A. Yagaub2, Einas M. Yousif2, Alaa I. Abdalla2, Rawan A. Elamin2, Howina S. Fadol2, Afra A. Fadl Alla2, Mohamed A. Hassan2 1Faculty of Pharmacy, University of Khartoum, Sudan 2Department of Biotechnology, Africa City of Technology, Khartoum, Sudan 3Department of Clinical Chemistry, Omdurman Islamic University, Sudan *Corresponding Author: [email protected] Abstract Background: TAL1 is a proto-oncogene whose distorted modifications in committed T-cell Precursors is related with the development of T-ALL, it also found to be related to many other human hematological diseases such as lymphoblastic lymphoma, immunodeficiency 18, acute myeloid leukemia and diamond-blackfan Anemia. Objectives: This study aims to predict the effect of nsSNPs on TAL1 protein structure function Methods: Retrieved nSNPs in the coding and 3’UTR regions were analyzed using different in silico tools. Interactions of TAL1 with functionally similar genes were investigated using Genemania. Post-translational modifications in several sites of the protein were also investigated. Results: Out of ninety nsSNPs identified, only eight were found damaging to protein function of which one is located in the basis helix-loop-helix domain (bHLH).
    [Show full text]