Qatar Foundation Annual Research Forum Volume 2010 Issue 1
- تاريخ المؤتمر: 12-13 Dec 2010
- الموقع: Qatar National Convention Center (QNCC), Doha, Qatar
- رقم المجلد: 2010
- المنشور: ١٣ ديسمبر ٢٠١٠
61 - 80 of 166 نتائج
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Gender differences in body composition, inflammatory markers and risk of metabolic abnormalities in Arabs
المؤلفون: Abdulaziz Farooq, Wade Knez, Asma Al Nuiami, Bengt Saltin, Vidya Mohamed-Ali and Justin GranthamAbstractBackground:Metabolic syndrome may be a result of both increased and/or inappropriate fat accumulation. As a consequence of the obesity epidemic, which has particularly manifested amongst the populations of the Arabian Gulf, associated with increases in type 2 diabetes mellitus and cardiovascular diseases, metabolic syndrome is becoming an increasing problem. Recent studies from the Gulf region have highlighted that women are more at risk than men. The effect of gender on fat accumulation and distribution, as well as its secretory function, are yet to be studied.
Purpose:The aim of our study was to investigate gender differences in body composition, aerobic fitness, adipokines and inflammatory markers in a cohort of healthy Qatari adults.
Methods:This was a prospective case-control study of healthy Qatari adults (18-50 years of age), comprised of 29 women matched with 29 men for age and body mass index. Detailed investigations included body composition by anthropometric measurements, DXA and CT scans to assess total and regional fat distribution. Subjects were also evaluated for their aerobic fitness and indices of muscular strength. Hematological investigations included fasting glucose, insulin, HOMA-IR, lipid profile analysis, adipokines (s-adiponectin, leptin) and inflammatory markers (IL-6, MCP-1, CRP, S.RANTES).
Results:Waist circumference in males (95.4±17.4 cm) and females (90.1±11.3 cm) was comparable (p=0.192). CT scan results revealed that women accumulate comparatively more fat in the total abdominal (p=0.036), and abdominal sub cutaneous (p=0.066) and total thigh (p<0.001) regions. No differences were detected in HOMA-IR, and despite very high adiposity, the lipid profile was favorable in females (TG=0.8±0.4 vs. 1.2±0.5 mmol/L and LDL=2.8±0.7 vs. 3.2±0.9 mmol/L). Poor aerobic fitness (<50th percentile) was observed in both groups 96% in women compared to 70% in men (p<0.001). S-adiponectin and leptin levels were significantly elevated in females, whereas CRP, IL-6, MCP-1 or S.RANTES were no different.
Conclusion:Elevated leptin concentration in women was attributed to a high percentage of central obesity in the test subjects. The presence of higher levels of s.-adiponectin led to a favorable lipid profile in women. In contrast, deleterious gender differences in aerobic fitness within this population is of critical relevance and must be further investigated.
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Novel poly (diol-co-tricarballylate) biodegradable elastomers. What makes them excellent carriers for controlled drug delivery and tissue engineering applications?
المؤلفون: Husam Mohammed Younes and Mohamed ShakerAbstractIn the past decade, biodegradable elastomeric polymers have gained considerable attention due to the renewed interest in their applications in the fields of biomedical tissue engineering and implantable drug delivery systems. Elastomers can be regarded as one of the best biomaterials for such applications because their mechanical properties can be manipulated in a manner that makes them as soft as body tissues, they have the ability to recover and withstand the mechanical challenges upon implantation in a mobile part of the body and they have also proven to be well suited to drug controlled drug delivery applications.
Our lab has recently reported on the successful preparation and characterization of a novel family of poly (diol-co-tricarballylate) elastomers, using visible light photo initiated polymerization. This new patented family of elastomers possess many structural, mechanical and physicochemical properties that make them superior to the currently available biodegradable elastomers.
The purpose of this presentation is to shed light on the preparation, characterization and in vivo animal biocompatibility studies conducted on these new elastomers. In addition, a short illustration on their application in controlled drug delivery and tissue engineering and the current and future scope of work planned utilizing the latest Qatar National Research Fund – National Priorities Research Program 3rd cycle support received will also to be presented.
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Factors influencing breast cancer screening practices among Arab women living in the State of Qatar
AbstractBreast cancer is frequently diagnosed in Arab women living in Qatar. Al Amal Hospital in Doha reported that 20% of cancer cases receiving treatment in 2007 involved the treatment of breast cancer among women. Early detection and treatment can reduce breast cancer morbidity and mortality rates significantly. However, Arab women are often diagnosed at advanced stages of breast cancer. Funded by the Qatar National Research Fund - National Priorities Research Program, we are undertaking a three-phase research program for which the goals are; (1) to understand the breast health experience of Arab women in Qatar, (2) identify and implement strategies that assist women to participate in breast cancer screening activities, and (3) evaluate, facilitate, and sustain the participation of Arab women in breast cancer screening. In phase I of the research program we will conduct two studies.
Study 1:This quantitative cross-sectional survey will investigate the participation rate of Arab women in breast cancer screening, their knowledge about breast cancer, barriers and facilitators to participation. Using a structured questionnaire, we will conduct face-to-face interviews with Arab women aged 35 and over in three different cities in Qatar (Doha, Al Wakrah, and Al Khor). Convenient sampling will be used to recruit 753 participants. Descriptive and inferential statistics will be performed using SPSS.
Study 2:This qualitative study will gain insight on; 1) how Arabic women view and participate in breast cancer screening activities, 2) how social, cultural, historical, and economic influences affect breast cancer screening for Arab women, the access to screening services, and social support networks in place, and 3) what intervention strategies will increase awareness of early detection and participation in breast cancer screening among Arab women. Purposive sampling will be used. Qualitative in-depth interviews will be individually conducted with Arab women, men, and healthcare providers. Qualitative data analysis will be performed. Although the results are not available at the present time, we will discuss how the information obtained from both the quantitative and qualitative studies will be used to develop culturally appropriate and effective intervention strategies and services to meet the preventative care needs of Arab women living in the State of Qatar with the aim of decreasing the seriousness and prevalence of breast cancer among them.
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Screening for and cloning and molecular characterization of two new oligopeptidase B encoding genes
المؤلفون: Fatma Baoumi Rashidi, Hatem El Shanti and Sayed GodaAbstractOligopeptidase B (opdB, EC 3.4.21.83) is a member of the prolyl oligopeptidase family of serine peptidases and unrelated to the trypsin and subtilisin families. It is a potential processing enzyme of prokaryotes to produce biologically active products, being very specific for the basic amino acid pairs of polypeptides. Bacterial oligopeptidase B cleaves globular proteins, albeit in a highly restricted fashion. While most members of this peptidase family hydrolyse peptide bonds at the C-terminal side of proline residues, oligopeptidase B exhibits a trypsin-like substrate specificity, cleaving peptides after basic residues (arginine or lysine). Oligopeptidase B was first cloned and characterized from Escherichia coli, and has also been described in other prokaryotes. Similar enzymes have been found in plants and some other higher organisms. We report the isolation of two different new oligopeptidase B bacterial strains producers. We identified the two genes, designated opdB1 and opB2. The opdB genes encodes a 703-residue peptide with high homology to the oligopeptidase B family in prokaryotes. The isolated opdBs gave the highest similarity score to oligopeptidase B of Stenotrophomonas maltophilia strain K279a (GenBank AM743169). To reveal the structural and kinetic properties of oligopeptidase B in more detail, we have cloned, expressed, and purified the enzymes to produce sufficient material to help in physical investigations, including NMR and x-ray crystallographic measurements. We also carried out a molecular characterization study of the two enzymes.
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Potential role of inositol 1,4,5 - triphosphate receptors in the pathogenesis of hypertension
المؤلفون: Abou Saleh Haissam, Shirley Haun, Nancy Rusch and Khaled MachacaAbstractInositol 1,4,5-triphosphate receptors (IP3R) are tetrameric intracellular channels that mediate the release of Calcium (Ca2+) from sarcoplasmic reticulum (SR) into the cytosol in response to IP3 binding. Modulation of vascular smooth muscle cells (VSMC) contractility allows small arteries to regulate blood flow and determine peripheral vascular resistance and blood pressure levels. The level of contraction of VSMC relies on a rise in cytoplasmic Ca2+ mediated by IP3-dependent Ca2+ release and voltage dependent Ca2+ influx through L-type Ca2+ (CaL) channels. Strong evidence supports a role for the vascular CaL channels in hypertension but little is known about the functional role of IP3R including the modulation of IP3R-Ca2+ signaling by the vascular endothelium. The goal of this study is to elucidate the functional contribution of IP3R-Ca2+ signaling to the pathogenesis of hypertension. Our preliminary results showed that IP3R are up regulated in small mesenteric arteries of two different forms of hypertensive rats. In the same arteries, activation of IP3R results in accentuated vasoconstriction whereas the endothelium-derived nitric oxide exerts a tonic dilator influence. The findings of this study will greatly improve our basic understanding of the etiology of hypertension by defining the abnormalities of IP3-dependent Ca2+ signaling and contraction in VSMC and its regulation by the endothelium. This may provide critical insights into the pathogenesis of hypertension, and set the groundwork for developing novel therapeutic strategies for the treatment of hypertensive disease.
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Molecular characterization and structure determination of human ADAMTSL4
المؤلفون: Yasmin Walid Abu aqel, Abdulghani Kohilan, Hatem El Shanti and Sayed Kamel GodaAbstractThe thrombospondin type 1 repeat (TSR) is an ancient extracellular protein domain that is commonly found in invertebrate and vertebrate proteins. The ADAMTSL4 protein, also known as TSRC1, belongs to the TSR superfamily and has multiple thrombospondin repeats, most of which are clustered at the C-terminus.
It has been reported that some TSP1 domain-containing proteins, e.g. thrombospondin 1 and thrombospondin 2, could induce apoptosis of endothelial cells but it is not clear how these proteins operate in death pathways.
Our recent work shows that mutations in ADAMTSL4 are responsible for autosomal-recessive isolated ectopia lentis, i.e. abnormal positioning of the lens of the eye and affect the development of the zonular fiber. However, little is known about the function of ADAMTSL4. To shed more light on the function of the ADMTSL4 and its roles in different tissues we extended our work to carry out molecular characterization of this gene and its variants.
We have obtained cDNA clones encoding the full ADAMTSL4 protein and its truncated isoform. Both are subcloned into the pET28a vector for expression in E. coli. In anticipation of possible expression challenges in this host, e.g. formation of inclusion bodies or lack of expression, we subcloned each fragment into the yeast vector, pYES2. The gene in both cases has been fused in frame with a region encoding an N-terminal His-Tag to facilitate the purification of the recombinant protein. DNA analysis indicates that each fragment has been correctly cloned into the pYES2 vector. Each construct was transformed into Saccharomyces cerevisiae for protein expression. Our preliminary analysis indicates that one of the genes is expressed in S. cerevisiae but at a very low level. Work to optimize the expression of ADAMTSL4 in yeast as well as in E. coli is in progress.
We also extracted the seven domains of the ADAMTSL4 using PCR. Each domain was subcloned into the E. coli overexpression vector, pET28a. Expression studies of all the constructs have shown that the seven domains have been successfully overexpressed in E. coli. The overexpression was confirmed using Western blot techniques. The recombinant protein of each domain is purified for NMR and x-ray studies.
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The impact of interventions on HIV transmission among couples in sub-Saharan Africa
المؤلفون: Hiam Chemaitelly and Laith Abu RaddadAbstractBackground:In areas highly endemic with HIV, discordancy is prevalent among couples affected by HIV, where a substantial proportion of infected individuals are in stable sexual relationships with non-infected individuals. Designing a package of interventions to reduce HIV incidence among discordant partnerships is critical. We assessed quantitatively the impact of four interventions (antiretroviral therapy (ART), pre-exposure prophylaxis (PrEP), condoms with and with no access to couple-based voluntary counseling and testing program (VCT), and male circumcision (MC)) on HIV incidence among a cohort of discordant couples at varying levels of efficacy, adherence, eligibility, and coverage.
Methods:A mathematical model was constructed to assess the impact of interventions and was parameterized by the best available evidence from clinical trials and observational studies. Uncertainty analyses were also conducted.
Results:Assuming full eligibility and coverage, ART, PrEP, condoms with (and with no) access to couple-based VCT, and MC reduced HIV incidence rate over three years by 69%, 37%, 36% (4.3%), and 19% respectively. Combining two interventions at a time led to a range of incidence rate reduction of 22%-82%; while combining three interventions led to a range of 76%-89%. Combining all four interventions reduced incidence rate by 92%. However, assuming realistic levels of eligibility, coverage, and adherence; ART, PrEP, condoms with (and with no) access to couple-based VCT, and MC reduced HIV incidence rate by 34%, 15%, 36% (2.3%), and 10%, respectively. An intervention package with two (three) interventions simultaneously reduced incidence rate between 12%-59% (24%-66%) depending on the eligibility and coverage conditions. Combining all 4 interventions reduced the incidence rate by 71%.
Conclusions:Despite substantial biological efficacy, the impact of each individual intervention is diluted at realistic levels because of eligibility, coverage, and adherence. However, combining multiple interventions can lead to large reductions in HIV incidence rate. ART is especially effective if combined with at least one other intervention and administered at intermediate to high levels of eligibility, coverage and adherence.
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Polymorphism in adiponectin receptor gene type 1 (ADIPOR1) in individuals with coronary artery disease with and without type 2 diabetes in the state of Qatar
المؤلفون: Nasser Mostafa RizkAbstractBackground:Previous studies demonstrated polymorphisms of adiponectin receptor type1 (AdipoR1) as a strong determinant of coronary artery diseases (CAD) susceptibility in type 2 diabetes. The aim of the study is to investigate the associations of the genetic marker (SNP) no of AdipoR1 locus; rs10920531 with CAD in patients with and without type 2 diabetes in the population of Qatar.
Methods:Blood was drawn from a total of 189 subjects. For the detection of the SNP (rs10920531, and rs7539542), extracted DNA was carried out by the 5′ nuclease assay using TaqMan MGB probe by means of an ABI 7900 [Applied Biosystems].
Results:Both groups of CAD, with and without diabetes mellitus (DM) had insignificant difference within the following parameters; age, BMI, glucose, lipid profile, cardiac enzyme markers, insulin and adiponectin. Females were 8.4% of all studied patients. The odds ratio and the frequency distribution of the genotype (rs1092531, A>C) revealed that (35.1%), [35.8%], had AA and (41.5%), [41.1%] had AC, and (23.4.0%), [23.1%] had CC among in control and cardiac patients with and without DM, respectively with P value=0.94. The odds ratio was 1.02 and 95% CI was (0.85-1.43). The frequency distribution of the genotype (rs7539542, C>G) revealed that (34.0%), [41.1%], had CC and (47.9%), [34.7%] had CG, and (18.1.0%), [24.2%] had GG among control and cardiac patients with and without DM, respectively with P value=0.37. The odds ratio was 0.98 and 95% CI was (0.65-1.47). The odds ratio was 0.77 for rs1092531, A>C and 0.92 for rs7539542, C>G among cardiac patients with and without diabetes. Using logistic regression analysis, LDL-C was significantly associated with both rs1092531, A>C and rs7539542, C>G in CAD patients. Hypertension was significantly associated with rs7539542.
Conclusion:No significant association was found between AdipoR1 locus; (rs1092531, A>C and rs7539542, C>G) and the cardiovascular disease (CVD) risks. Of all CVD risks, Only LDL-C correlated significantly with (rs1092531, A>C and rs7539542, C>G). Hypertension was significantly associated with s7539542. Further studies are needed among the Qatari population to screen polymorphisms of the entire diponectin gene and its receptors.
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The spectrum of Mediterranean fever (MEFV) mutations in an Arabic cohort
AbstractAutoinflammatory diseases are a group of disorders characterized by seemingly unprovoked inflammation in the absence of high-titer autoantibodies or antigen-specific T cells. Familial Mediterranean fever (FMF) is an autosomal recessive disorder and the archetypal autoinflammatory disease. It is characterized by recurrent self-limiting episodes of fever and painful polyserositis. FMF is prevalent in specific ethnic groups namely, non-Ashkenazi Jews, Armenians, Turks, and Arabs. The gene responsible for FMF, MEFV, was identified in 1997. There seems to be a distinctive clinical picture in Arab patients with FMF, and the range and distribution of MEFV mutations is different from that noted in other commonly affected ethnic groups.
The aim of this study was to delineate the distribution of MEFV mutations amongst an Arabic FMF patient cohort and to assist the genotype-phenotype correlation in these patients. We collected DNA samples from 406 FMF patients (from Qatar, Jordan, Algeria and Palestine) who have been clinically diagnosed with FMF. We designed primers to cover the entire genomic region of MEFV. Mutation detection is done by resequencing the entire coding sequence and splice sites then the rest of the genomic region and the promoter will be sequenced as a second tier.
So far we have identified 283 (out of 676) mutant alleles by sequencing exon 10, the main hot spot for MEFV mutations (M694V, V726A, M694I, M680IGC, M680IGA, R653H, A744S and R761H). In addition, four novel variations were identified in our cohort in exons 3, 5, 2 & 10, and we are currently investigating the phenotypic significance of these novel variations.
The spectrum of MEFV mutations in Arabs seems different from other ethnic groups commonly affected by FMF. The identifiable disease causing alleles are the lowest amongst the commonly affected ethnic groups. The low number of identified alleles suggests the presence of mutations within unexamined regions, such as conserved intronic sequences or the involvement of modifier genes.
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Metal toxicity at the synapse: presynaptic, postsynaptic and long-term effects
المؤلفون: Zena Basil Ghazala, Sanah Sadiq, Arnab Chowdhury and Dietrich BüsselbergAbstractMetal toxicity is a global health concern. We summarize the evidence for metal interactions with the nervous system with an emphasis on synaptic transmission. The appropriate functioning of synaptic transmission is crucial for the information transfer in any neural network.
Presynaptically, metal ions modulate transmitter release through their interaction with neurotransmitter (NT) synthesis, fusion of synaptic vesicles, signaling cascades and ion channels. Ca2+ entry through voltage-gated channels is impaired by Pb2+, Cd2+ or Zn2+, therefore all processes which depend on Ca2+, including NT release, will be affected. Furthermore, some metals interact with intracellular pathways e.g. Pb2+ inhibits PKC enzymes through its catalytic domains, and Ni2+ causes a decline in the transcription of two isoforms of PKC (prkcc and prkz) and two regulatory binding proteins (prkcbp1 and prkcdb) affecting most functions of PKC. Cd and Hg inhibit adenylate cyclase activity, while the extent of inhibition depends on exposure time and brain area. Exocytosis is impaired by Pb2+ and Cu2+, which interact with Synaptotagmin I.
Postsynaptically, processes associated with binding of NT to their receptors, activation of the channels and degradation of NT are changed by metal. Zn2+, Pb2+, Cu2+, Cd2+, Ni2+, Co2+, Li3+, Hg+ and methylmercury modulate NMDA, AMPA/Kainate and/or GABA receptor's activity. These effects are more or less specific e.g. Zn2+ and Cu2+ modulate all three types of receptors, while Zn2+ is more potent (IC50= 0.77μM) compared to Cu2+ (IC50=15μM) at NMDA-Rs, but both have similar potencies at GABA-R. For the most part, metal interactions depend on the subunit composition of the NMDA-R, while less data are available for other targets, possibly underestimating their importance.
These modulations change the synaptic efficiency and therefore impair long-term potentiation (LTP). Consequently, metals such as Al, Pb or Cd result in various cognitive deficits. In addition the generation and maintenance of LTP is reduced by metal actions on phosphorylation of transcription factors like CREB as well as by reduction of nitric oxide synthase (NOS) that change retrograde signaling.
Overall, there are multiple effects of metals based on the forms of the metals, their concentrations and the types of neurons involved.
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Analysis of cortical development in Lis1-GFP mice
المؤلفون: Khawla Fuad Ali and Anamaria SudarovAbstractThe Lis1 gene encodes a non-catalytic sub-unit of the platelet-activating factor acetyl hydrolase enzyme (PAFAH1B1). Increased PAFAH1B1 dosage in humans causes mild brain structural abnormalities, moderate to severe developmental delay and failure to thrive. To investigate the effects of Lis1 over expression on cortical development, we analyzed the brains of Lis1-GFP mice with 30% over expression in the Lis1 gene.
Cortical width was thinner for Lis1-GFP mice than for wild type at embryonic day 14.5 (E14.5), post-natal day 1 (P1) and P6 but appeared to be similar at P120. Analysis of cell proliferation at E14.5 showed a reduction in rates of proliferation at the ventricular zone (VZ) of Lis1-GFP mice compared to wild type. As a result, less Pax6-positive cells of the VZ were seen at P1 in the Lis1-GFP mice. Immunostaining for pyramidal neuron marker Brn2 showed cellular disorganization within the upper cortical layers (layers II and III) of P1 mice, while other layers (I, IV, V and VI) appeared to form properly. Analysis of cortical plate formation and laminar structure via BrdU birth-dating at P1 and P21 showed successful radial migration of neurons born at the VZ at ∼E12.5 and ∼E14.5 to their final destined layer. Disorganization of layers II and III was also seen in BrdU birth-dating analysis, and that supported our Brn2 findings. The number and density of mature neurons was assessed in the cerebral cortex of adult Lis1-GFP mice (P120). Numbers and densities were similar in all cortical layers between Lis1-GFP mice and wild type, except for layers II and III which showed significant reduction in neuronal count. Quantification of GABAergic interneurons within the six cortical layers of P120 mice revealed no significant difference between wild type and Lis1-GFP mice.
Collectively, our results show that Lis1 over expression in the Lis1-GFP mice results in decreased proliferation rates of neuronal progenitors at the VZ pre-natally. Subsequently, this may interfere with the proper formation of upper cortical layers (layers II and III) in young and adult Lis1-GFP mice.
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Regulation of store-operated channels by endoplasmic reticulum chaperons
المؤلفون: Mashael Al-Shafai, Abdelilah Arredouani, Hamid Mesaeli, Nasrin Mesaeli and Khaled MachacaAbstractCalreticulin is a conserved Ca2+ binding chaperone protein that is localized to the lumen of the endoplasmic reticulum (ER). The protein is implicated in many cellular functions such as the regulation of intracellular Ca2+ homeostasis, the regulation of gene expression, the folding of the newly synthesized proteins, cell adhesion, cancer and auto-immunity. The role of calreticulin in Ca2+ homeostasis regulation through Ca2+ storage and signaling might be the key to explaining the involvement of the protein in many biological functions inside and outside the ER. In this study, we examined whether calreticulin is responsible for regulating store-operated channels (SOC) on the plasma membrane by assessing changes in Ca2+ levels and SOC activity in mouse embryonic fibroblasts that are deficient in calreticulin. Wild type and calreticulin deficient fibroblasts were loaded with fura2-AM and the release of Ca2+ from the ER stores was induced using Thapsigargin or Ionomycin, and Ca2+ levels were measured using InC lm2 computer program. Calreticulin-defiecint fibroblasts showed a marked decrease in Ca2+ influx through SOC compared to wild type. To investigate the mechanism that underlines this decrease in SOC activity we performed western blots using antibodies for ORAI (Calcium release-activated calcium channel protein) and STIM (stromal interacting molecule). Our data showed a significant decrease in the expression of ORAI in the calreticulin-deficient fibroblasts compared to wild type while STIM expression in calreticulin-defiecint fibroblasts did not significantly differ from wild type. We concluded from our data that calreticulin controls SOC activity and this seems to be through regulating the expression of ORAI on the plasma membrane.
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Tumor associated mesenchymal stem cells protect ovarian cancer cells from hyperthermia through CXCL12
المؤلفون: Fadwa Ali, Arash Rafii, Raphael Lis and C TouboulAbstractHyperthermic intraperitoneal chemotherapy (HIPEC) has shown promise in the treatment of ovarian carcinosis. Despite its efficiency for the treatment of peritoneal carcinosis from digestive tract neoplasia, it has failed to demonstrate significant benefit in ovarian cancers. It is therefore essential to understand the mechanism underlying the resistance to HIPEC in ovarian cancers. Mesenchymal Stem Cells (MSC) play an important role in the development of ovarian cancer metastasis and resistance to treatments. A recent study suggests that MSCs may be cytotoxic for cancer cells upon heat shock. In contrast, we describe the protective role of MSC against hyperthermia. Using cytokine arrays we determined that tumor associated MSC (TAMC) secrete pro-tumoral cytokines. We studied the effect of hyperthermia in co-culture setting of TAMC or bone marrow derived-MSC (BM-MSC) associated with ovarian cancer cell lines (SKOV3 and CaOV3) with polyvariate flow cytometry. We demonstrate that hyperthermia does not challenge survival of TAMC or BM-MSC. Both TAMC and BM-MSC displayed strong protective effect inducing thermotolerance in ovarian cancer cells (OCC). Transwell experiments demonstrated the role of secreted factors. We showed that CXCL12 was inducing thermotolerance and that inhibition of CXCL12/CXCR4 interaction restored cytotoxicity of hyperthermia in co-culture experiments. Targeting the interaction between stromal and cancer cells through CXCL12 inhibition might restore hyperthermia sensitivity in ovarian cancers, and thus improve HIPEC efficiency.
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Initial investigation of ubiquitination pathway in mammalian meiosis
المؤلفون: Amna Mohammed Al-Khuzaei and Paula CohenAbstractThe Cohen's lab research focuses mainly on the regulation of mammalian meiosis in mouse models, which include several induced mutants that have helped in broadening our knowledge of meiotic recombination and the gametogenesis. The lab also studies several DNA mismatch repair (MMR) proteins and their subsequent effects on meiotic recombination. Thus, our research serves two major purposes; first, to understand the genetics of re-combination and thereby to understand how such events can fail in human gametogenesis and secondly, to further elucidate the mechanisms of DNA repair and genome stability in an important in vivo system.
Extending from these aims, one of these genes is the MLH3 gene, evolutionarily conserved in many species such as mice, humans, and worms and which can solve the infertility problems in MLH3 mutant mice.
The focus of our project is to investigate the functions of several genes involved in meiotic prophase, using the technique of chromosome spreading. This method allows us to visualize the different stages of prophase I, and see the staining pattern of several antibodies that are specific to meiotic proteins. Using a battery of specific antibodies, we set out to understand the meiotic roles of a number of poorly characterized proteins involved in DNA repair and ubiquitination pathways. These antibodies of interest are those that are involved in the ubiquitination pathway of the sex chromosomes such as antibodies raised against Rnf 8, Rad 18, and Rnf 168, all of which are involved in ubiquitination pathways, as well as other antibodies involved in ubiquitination/deubiquitinatio. A group of other antibodies that include mdc λ, HR9B, MRαB, USP2B, and UBQ 2 is also being studied. Our goal was to first characterize the accumulation of these proteins on meiotic chromosomes in order to identify which, if any of these proteins might be functionally relevant for meiotic recombination and prophase | progression.
The project started with studying the staining pattern of the antibodies listed above in adult male wild type mice, then younger male wild type mice to see both the early and late stages of meiosis. The project is progressing to studying the staining pattern in the MLH3 and Ago 4 mutant mice to see any possible co-localizations between MMR genes and the antibodies considered by this study
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Gene identification in Mendelian forms of familial epilepsy
المؤلفون: Hala Mint El Moctar, Mohamed El Dow, Yasser Al Saraj, Jamil Alami and Hatem El ShantiAbstractEpilepsy encompasses a heterogeneous group of recurrent seizure disorders affecting 1% of the world's population. Idiopathic generalized epilepsy accounts for 40% of all epilepsy disorders. Genetic factors contribute significantly to the etiology of idiopathic generalized epilepsies. Complex non-Mendelian forms of familial epilepsies comprise the majority of idiopathic generalized epilepsies, where susceptibility genes remain largely unknown. However, rare Mendelian or monogenic familial epilepsies have contributed to our understanding of the genetic heterogeneity and complexity of epilepsy disorders. Recent advances in the genetics of epilepsy have identified most monogenic idiopathic generalized epilepsies as being caused by various channelopathies of which the majority show an autosomal dominant pattern of inheritance. In this study we aim to identify gene(s) responsible for autosomal recessive forms of familial idiopathic generalized epilepsy.
We identified one consanguineous family with idiopathic generalized epilepsy showing an autosomal recessive pattern of inheritance. Age of onset of epilepsy in affected family members was in early adolescence. The majority manifest generalized tonic-clonic seizures and abnormal EEG findings. We performed whole-genome single nucleotide polymorphism genotyping for the five family members using Illumina platform (200,000 single nucleotide polymorphisms). Linkage analysis by homozygosity mapping (Homozygosity Mapper) was performed.
We identified one region spanning approximately10 Mb on the long arm of chromosome 11. The region contains 279 protein-coding genes. Candidate genes were prioritized in-silico based on brain expression and conservation through evolution. The identified candidate genes are re-sequenced (Sanger sequencing, big dye terminator chemistry) and one gene has been excluded up to date. We are currently re-sequencing and pre-forming mutation analysis on the remaining ten candidate genes.
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Role of mesenchymal stem cells in enhancing ovarian cancer metastasis
المؤلفون: Hamda Al-Thawadi, Rafael Lis, C Touboul, C Raynaud and Arash RafiiAbstractCancer accounts for the death of thousands of people each year and brings pain and suffering to thousands more. Among cancers that specifically affect women, ovarian cancer has the highest fatality rate as 7 out of 10 women die within 5 years of surgery. As highlighted in numerous recent publications, the role of the microenvironment in the development and progression of cancer is critical, albeit not entirely understood and should therefore be a focal point for further inquiry. The goal of our study was to define the metastatic properties enhanced by the interaction between ovarian cancer cells and mesenchymal stem cells. We studied the interaction between ovarian cancer cells and mesenchymal stem cells (MSC) using two different ovarian cancer cell lines (OVCAR3 and SKOV3) as well as different MSC cell lines derived from specific tissue. We studied using cytokine array as well as kinase array the modifications of the MSC upon their interaction with ovarian cancer cells. We demonstrated increased expression of cytokines that might be implicated in ovarian cancer metastasis (IL6 and IL8). Moreover MSC helped the ovarian cancer cells to grow in a tri-dimensional cell culture system. Finally we were able to define transcriptomic modification in the MSC and ovarian cancer cells upon their interaction.
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Enhanced EGFR expression and function in calreticulin deficient cells
المؤلفون: Amit Abraham, Hanin Abou Ayash, Hala Omar, Hamid Massaeli and Nasrin MesaeliAbstractIntroduction:Calreticulin is a multi-functioning protein located in the endoplasmic reticulum. Several functions have been attributed to calreticulin including lectin-like chaperoning, regulation of gene expression, cell adhesion, auto-immunity and calcium homeostasis. As an endoplasmic reticulum chaperone calreticulin regulates the maturation and folding of several trans-membrane proteins. We hypothesized that as an endoplasmic reticular protein it regulates the expression folding and maturation of epidermal growth factor receptor (EGFR). To date no information is available about the role of calreticulin in EGFR expression and folding.
Methods:Wild type calreticulin deficient (crt -/-) and mouse lung cancer cells isolated from transgenic mice over expressing calreticulin was used to examine the expression, localization and function of EGFR. Western blot analysis was used to determine the protein expression. Immunocytochemical staining of cells was utilized to determine localization of EGFR and AKT phosphorylation was used to determine changes in EGFR function.
Results:Loss of calreticulin function resulted in a significant increase in the expression of EGFR as was determined by western blot analysis with anti-EGFR antibody. Similarly, lung tumor cell lines isolated from calreticulin over expressing cells expressed high levels of EGFR. Immunocytochemical staining of these cells did not show any significant change in the localization of EGFR in either calreticulin deficient or over expressing cells.
Our data also demonstrated an increase in the level of tyrosine phosphorylation in calreticulin deficient cells accompanied by a significant increase in the AKT phosphorylation in these cell lines suggesting an increase in EGFR activity.
Conclusions:Altered calreticulin expression does not affect EGFR receptor folding but rather increases its expression and function. Next we will examine whether changes in the EGFR is due to calreticulin's role as a regulator of intracellular calcium thus affecting transcription of EGFR (using quantitative RT-PCR technique).
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Label-free intrinsic imaging capillary zone electrophoresis analysis to detect homocysteine from blood serum for the detection of genetic metabolic disorders in new-born babies in Qatar
المؤلفون: Amira Khalaf AljabiryAbstractOver 14,000 babies are born in Qatar each year, and it is the State's intention to provide each with a health screen at birth for the timely diagnosis of inborn errors of metabolism. And since the population is characterized by a high consanguinity (estimates vary between 25–70%) from first-cousin marriages, congenital and genetic disorders are responsible for a major proportion of infant mortality, morbidity, and handicap birth defects and are relatively common among the population. Accurate and reliable quantification of amino acid (AA), generally in a plasma sample, allows early diagnosis of disorders such as phenylketonuria, tyrosinemia, maple syrup urinary disease, hyperornithinemia and citrullinemia. A deficiency of cystathionine B-synthase (CBS) can cause an autosomal recessive disorder of methionine and homocysteine (Hcy) metabolism known as homocystinuria which results in elevated concentrations of Hcy in plasma and urine. Clinical symptoms in untreated patients include progressive myopia and lens dislocation, thromboembolism, epilepsy, and mental retardation. Hcy is implicated as a wide variety of natal and other disorders – including Alzheimer's. The aim of this study is to develop novel screens for AA levels – and in particular Hcy - in the blood using novel approaches in capillary zone electrophoresis (CZE). In order to quantify relevant amino acids it is necessary to deplete proteins from a complex biological sample such as plasma. In this investigation two protein depletion protocols were investigated on human plasma containing Hcy by label-free intrinsic imaging in the UV using CZE. As with a majority of amino acids, Hcy has very little or no UV absorption and for this reason analysis of samples were performed on an advanced high performance capillary electrophoresis (HPCE) platform, by multiple-pixel multiple-imaging indirect UV measurements. Two complementary analysis workflows were deployed to take advantage of the time-development of the AAs in the analysis allowing accurate quantification and minimum inherent bias.
Studies have been made with pure AAs and also with samples spiked in known quantities in blood which offer real clinical advantages. We have also developed methodologies for the simultaneous detection of several amino acids in plasma samples and limits of detection (LOD) and limits of quantification (LOQ) will be presented. These have been shown to be greatly improved with a pre-concentration technique known as ‘stacking’. Work has been undertaken in our labs in Qatar Science & Technology Park and in collaboration with Hamad Medical Center.
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Calreticulin mediated control of polycystin-2 expression
المؤلفون: Amit Abraham, Emine Turgut-Neary, Hala Omar, Hamid Massaeli and Nasrin MesaeliAbstractPolycystin-2 or transient receptor potential polycystic 2 (TRPP2) is a membrane glycoprotein that is encoded for by the gene pkd-2, which accounts for ˜15% of autosomal dominant polycystic kidney disease. TRPP2 is an independent non selective cation channel localized to either the plasma membrane or the endoplasmic reticulum (ER) that is involved in diverse cellular functions including control of cell cycle, cell wall synthesis, left-right symmetry, cardiac & renal development and mating behavior. In addition, it interacts with polycystin-1 that regulates different cell signaling pathways including JAK/STAT. As a trans-membrane protein, polycystin-2 is expressed, folded and matured in the endoplasmic reticulum. To date no data is available about the nature of endoplasmic reticulum which is responsible for the proper folding of polycystin-2. This led us to the hypothesis that calreticulin, an endoplasmic reticular calcium binding chaperone protein, is involved in stabilizing and transporting polycystin-2 to the plasma membrane.
To test this hypothesis we examined changes in polycystin expression and localization in wild type and calreticulin deficient cells using western blot analysis, and immunocytochemistry. Furthermore, western blot and immunohistochemical analyses were used to examine changes in polycystin expression and localization upon calreticulin over expression in vascular smooth muscle and endothelial cells of transgenic mice.
Our data showed that over expression of calreticulin in either vascular smooth muscle cells or endothelial cells of transgenic mice results in the development of multiple clear cysts in the kidney cortex of these mice. Histopathological analysis of these kidneys resembles those of human polycystic kidney disease. Furthermore, loss of calreticulin function resulted in altered polycystin-2 expression in the mouse embryonic fibroblast cell lines. However, there were no significant changes in the localization of polycystin-2 protein in calreticulin deficient cells when compared to the wild type cells.
Our data supports a possible role for calreticulin in the expression of polycystin-2. Further research is warranted to elucidate the role of calreticulin as a chaperone or regulator of calcium homeostasis in the expression of polycystin-2.
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A new 3-dimensional model for ovarian cancer based on amniotic membrane
المؤلفون: Halema Al FarsiAbstractEpithelial ovarian carcinoma (EOC) is the sixth most common malignancy in women and the leading cause of death from gynecological cancer in the world. One of the main differences between ovarian cancers and other neoplasm is burden of local extension. Hence the majority of mortality in ovarian cancer is due to extensive peritoneal disease, with a high rate of mortality and an overall survival rate ranging from 20% to 30% five years after surgery according to various studies. As for any metastatic process, the tumor cells have to go through the steps of detaching from the primary tumor, adhering to the peritoneal surface and then invading the peritoneum. Each of these steps might be critical in the development of a metastatic lesion. Therefore it is essential to understand the molecular background of peritoneal adhesion and invasion in order to define new therapeutic targets. It may be that classic 2-dimensional cultures do not represent an ideal model for the initiation of metastasis, and therefore studies using only 2-dimensional cell cultures might not replicate the reality of ovarian cancer physiology. The goal of our study was to define new 3-dimensional culture models that will mimic the peritoneal tissue. The constraints were; to use an easily accessible tissue, in relevant quantities, as close as possible to the peritoneum, with great manipulability. We demonstrated that we could keep the amniotic membrane in culture and mimic adhesion and the early invasion of ovarian cancer cell aggregates. We were then able to follow the invasive process within the membrane and determine different cell behavior.
Developing reproducible 3-dimensional models of ovarian cancer aggregates and early adhesion and invasion will help us gain a more accurate understanding of the molecular mechanisms involved in the ovarian cancer metastatic process and define potential new therapeutic targets hindered by the use of classic 2-dimensional models.
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