Therapeutic Monoclonal Antibodies and Emergence of Their Biosimilars

en 29849980 Therapeutic Monoclonal Antibodies and Emergence of Their Biosimilars Antibodies are proteins of the immune system that are produced by B-lymphocytes. These proteins exert their effects by recognizing and binding to their targets (antigens). A monoclonal antibody (mAb) is originally produced by a single B-cell. Production of mAbs was first introduced in 1975 using cell fusion technique and hybridoma cell production. A Hybridoma is formed by fusion of an antibody producing B-lymphocyte and a myeloma cell line. These cells have two main characteristics, production of uniform, monospecific antibodies (mAbs) that originate from the B-cell and immortality that comes from the myeloma cell line. A hybridoma cell line is thus acting like a biological factory that produces and secretes mAbs into the cell culture medium. Most of the mAbs have been produced in mice and are thus proteins of murine origin. mAbs were later found to be able to bind biological targets like tumor antigens, molecules involved in autoimmune and infectious disease-related molecules, etc. This led to emergence of therapeutic monoclonal antibodies. However, since the first mAbs were murine proteins (OKT3 was injected to kidney transplant patients to prevent graft rejection), their repeated administration raised Human Anti Mouse Antibody (HAMA) in the patients that resulted in neutralization of the injected mAb (OKT3). The solution was to genetically change the murince antibodies to human antibodies. In this regard chimeric (%80 -%90 human), humanized (≥ %90 human) and fully human (%100 human) therapeutic mAbs were produced. At present more than 50 therapeutic mAbs are on the market with more than 120 billion USD global market share. These mAbs have shown very good therapeutic effect in treatment of cancers, autoimmune and infectious diseases. However, these drugs are very expensive and thus their patient accessibility is limited. Although, they are protected by patents, some patents have already expired and some are close to expiration dates. Here, biosimilar versions of these drugs have started to immerge. Biosimilars are defined as biological drugs that are highly similar but not identical to the biological reference (original or originator) drug. The approval of biosimilars to enter the biopharmaceutical market is governed by the regulatory bodies in different countries. This happens under strict and comprehensive comparability exercise. The biosimilarity determination procedure is planned to ensure that the difference between the originator and the biosimilar drug is not clinically significant. The assessment includes immunochemical and physicochemical properties, biological activity, structural similarity, purity, contamination with impurities like host cell protein and DNA. In addition, in vivo pharmacology studies like pharmacokinetic and pharmaco-dynamic characteristics as well as, efficacy, safety and tolerability must be determined and approved. Moreover, after market analyses like pharmaco-epidemiological studies should also be done. These procedures are also necessary to be performed to assure the prescribing physicians to suggest them to their patients. Thus, the biosimilars, due to their lower production costs, are expected to introduce huge amounts of cost savings to healthcare systems and more importantly, increase affordability/accessibility of biological treatment. 61 61 https://www.ajmb.org/En/Article.aspx?id=295 https://www.ajmb.org/PDF/En/FullText/295.pdf MahmoodJeddi-TehraniDepartment of Hybridoma, Monoclonal Antibody Research Center, Avicenna Research Institute, ACECR, Tehran, Iran15

en 29849981 Effects of Hypoxia on Biology of Human Leukemia T-cell Line (MOLT-4 cells) Co-cultured with Bone Marrow Mesenchymal Stem Cells Background: One of the most significant problems in the treatment of leukemia is the expansion of resistance to chemotherapeutic agents. Therefore, assessing the drug resistance and especially the drug resistance genes of leukemic cells is important in any treatment. The impact of Mesenchymal Stem Cells (MSCs) and hypoxic condition have been observed in the biological performance of majority of leukemic cells. Methods: MOLT-4 cells were co-cultured with MSCs in the hypoxic condition induced by Cobalt Chloride (CoCl2) for 6 and 24 hr. Then, apoptosis of cells was analyzed using annexin-V/PI staining and expression of the drug resistance genes including MDR1, MRP, and BCRP along with apoptotic and anti-apoptotic genes, including BAX and BCL2, was evaluated by real-time PCR. Results: The hypoxic condition for MOLT-4 cells co-cultured with MSCs could significantly increase the expression of MDR1 and BCRP genes (p<0.05) which are involved in drug resistance. Also, the results indicated that this condition significantly increases the expression of BCL2 (p<0.05) and reduces the apoptosis in MOLT- 4 cells co-cultured with MSCs in the hypoxic condition. Conclusions: These effects can demonstrate the important role of hypoxia and MSCs on the biological behavior of Acute Lymphoblastic Leukemia (ALL) cells that may lead to particular treatment outcomes. Acute lymphoblastic leukemia, Drug resistance, Hypoxia, Mesenchymal stem cell 62 68 https://www.ajmb.org/En/Article.aspx?id=312 https://www.ajmb.org/PDF/En/FullText/312.pdf SinaBaharaghdamHematology and Oncology Research Center, Tabriz University of Medical Sciences, Tabriz, Iran1246MehdiYousefiDepartment of Immunology, Faculty of Medicine, Tabriz University of Medical Sciences, Tabriz, Iran610Ali AkbarMovasaghpourHematology and Oncology Research Center, Tabriz University of Medical Sciences, Tabriz, Iran1072SaeedSolaliHematology and Oncology Research Center, Tabriz University of Medical Sciences, Tabriz, Iran1247MehdiTalebiHematology and Oncology Research Center, Tabriz University of Medical Sciences, Tabriz, Iran1248MiladAhani-NahayatiHematology and Oncology Research Center, Tabriz University of Medical Sciences, Tabriz, Iran1249HamidLotfimehrHematology and Oncology Research Center, Tabriz University of Medical Sciences, Tabriz, Iran1250KarimShamsasanjanHematology and Oncology Research Center, Tabriz University of Medical Sciences, Tabriz, Iran1251

en 29849982 The Evaluation of Astaxanthin Effects on Differentiation of Human Adipose Derived Stem Cells into Oligodendrocyte Precursor Cells Background: Multiple Sclerosis (MS) has been explained as an autoimmune mediated disorder in central nerve system. Since conventional therapies for MS are not able to stop or reverse the destruction of nerve tissue, stem cell-based therapy has been proposed for the treatment of MS. Astaxanthin (AST) is a red fat-soluble xanthophyll with neuroprotection activity. The aim of this study was evaluation of pre-inducer function of AST on differentiation of human Adipose- Derived Stem Cells (hADSCs) into oligodendrocyte precursor cells. Methods: After stem cell isolation, culture and characterization by flow cytometry, hanging drop technique was done for embryoid body formation. In the following, hADSCs were differentiated into oligodendrocyte cells in the presence of AST at various concentrations (1, 5, and 10 ng/ml). Finally, immunocytochemistry and real-time PCR techniques were used for assessment of oligodendrocyte differentiation.  Results: Flow cytometry results indicated that hADSCs were CD44, CD49-positive, but were negative for CD14, CD45 markers. In addition, immunocytochemistry results revealed that, in AST treated groups, the mean percentage of Olig 2 and A2B5 positive cells increased especially in 5 ng/ml AST treated group compared to control group (p<0.001). Moreover, real-time PCR analysis confirmed the results of immunocytochemistry. Conclusion: Since hADSCs have the potential to differentiate into multi lineage cells and due to important functions of AST in regulating various cellular processes, it seems that AST can be used as a promoter for oligodendrocyte differentiation of hADSCs for being used in cell transplantation in multiple sclerosis. Adult stem cells, Astaxanthin, Multiple sclerosis, Oligodendroglia 69 74 https://www.ajmb.org/En/Article.aspx?id=307 https://www.ajmb.org/PDF/En/FullText/307.pdf NazemGhasemiDepartment of Anatomical Science and Molecular Biology, Faculty of Medicine, Isfahan University of Medical Sciences, Isfahan, Iran1156

en 29849983 Ectopic Expression of Human DPPA2 Gene in ESCC Cell Line Using Retroviral System Background: Cancer/Testis Antigens (CTAs) are a subgroup of tumor-associated antigens which are expressed normally in germ line cells and trophoblast, and aberrantly in a variety of malignancies. One of the most important CTAs is Developmental Pluripotency Associated-2(DPPA2) with unknown biological function. Considering the importance of DPPA2 in developmental events and cancer, preparing a suitable platform to analyze DPPA2 roles in the cells seems to be necessary. Methods: In this study, the coding sequence of DPPA2 gene was amplified and cloned into the retroviral expression vector to produce recombinant retrovirus. The viral particles were transducted to Esophageal Squamous Cell Carcinoma (ESCC) cell line (KYSE-30 cells) and the stable transducted cells were confirmed for ectopic expression of DPPA2 gene by real-time PCR. Results: According to the critical characteristics of retroviral expression system such as stable and long time expression of interested gene and also being safe due to deletion of retroviral pathogenic genes, this system was used to induce expression of DPPA2 gene and a valuable platform to analyze its biological function was prepared. Transduction results clearly showed efficient overexpression of the gene in target cells in protein level due to high level of GFP expression. Conclusion: Such strategies can be used to produce high levels of desired protein in target cells as a therapeutic target. The produced recombinant cells may present a valuable platform to analyze the effect of DPPA2 ectopic expression in target cells. Moreover, the introduction of its potential capacity into the mouse model to evaluate the tumorigenesis of these cancer cells in vivo leads to an understanding of the biological importance of DPPA2 in tumorigenesis. In addition, our purified protein can be used in a mouse model to produce specific antibody developing a reliable detection of DPPA2 existence in any biological fluid through ELISA system. Carcinogenesis, Esophageal squamous cell carcinoma, Germ cells, Testis 75 82 https://www.ajmb.org/En/Article.aspx?id=305 https://www.ajmb.org/PDF/En/FullText/305.pdf MaryamKhaleghizadehHuman Genetic Division, Immunology Research Center, Avicenna Research Institute, Mashhad University of Medical Sciences, Mashhad, Iran1213Mohammad MahdiForghanifardHuman Genetic Division, Immunology Research Center, Avicenna Research Institute, Mashhad University of Medical Sciences, Mashhad, Iran1214AbolfazlRadCellular and Molecular Research Center, Sabzevar University of Medical Sciences, Sabzevar, Iran1215MoeinFarshchianHuman Genetic Division, Immunology Research Center, Avicenna Research Institute, Mashhad University of Medical Sciences, Mashhad, Iran1216ZahraHejaziDepartment of Microbiology, Damghan Branch, Islamic Azad University, Damghan, Iran1217MehranGholaminHuman Genetic Division, Immunology Research Center, Avicenna Research Institute, Mashhad University of Medical Sciences, Mashhad, Iran1218BahramMemarDepartment of Pathology, Imam Reza Hospital, Mashhad University of Medical Sciences, Mashhad, Iran1219Mohammad RezaAbbaszadeganMedical Genetics Research Center, Faculty of Medicine, Mashhad University of Medical Sciences, Mashhad, Iran1220

en 29849984 Lavandula angustifolia Effects on Rat Models of Alzheimer’s Disease Through the Investigation of Serum Metabolic Features Using NMR Metabolomics Background: Alzheimer’s Disease (AD) is the most prevalent cause of memory impairment in the elderly population, but the diagnosis and treatment of the disease is still challenging. Lavender aqueous extract has recently been shown to have the potential in clearing Amyloid-beta plaques from AD rat hippocampus. To elucidate the therapeutic mechanisms of lavender, serum metabolic fingerprint of Aβ-induced rat Alzheimer’s models was investigated through nuclear magnetic resonance spectrometry. Methods: For the establishment of rat Alzheimer’s models, 10 μg of Amyloid beta 1-42 was injected to male Wistar rats. The lavender aqueous extract was injected 20 days after the establishment of the models, once daily for 20 days. Serum samples were collected and metabolite fingerprints were obtained using 500 MHz 1H-NMR spectrometry, following multivariate statistical analyses. The resulted metabolites were then subjected to pathway analysis tools to reveal metabolic pathways affected by the lavender extract treatment. Results: Levels of 10 metabolite markers including alanine, glutamine, serine, isoleucine, valine, carnitine, isobutyrate, pantothenate, glucose and asparagine were reversed nearly to control values after treatment with lavender extract. The results revealed that the most significantly affected pathways during treatment with lavender extract belonged to carbohydrate and amino acid metabolism, including pantothenate and CoA metabolism, glyoxilate and dicarboxylate metabolism, alanine, aspartate and glutamate metabolism, cysteine and methionine metabolism. Conclusion: As lavender extract reversed the direction of changes of some metabolites involved in AD pathogenesis, it was concluded that the extract might play a role in the disease improvement and serve as a potential therapeutic option for the treatment of AD. Moreover, the metabolites which were found in AD rats could serve as a potential marker panel for the disease; however, much further investigation and validation of the results is needed. Alzheimer disease, Lavandula, Metabolomics, Serum 83 92 https://www.ajmb.org/En/Article.aspx?id=306 https://www.ajmb.org/PDF/En/FullText/306.pdf AfsanehArefi OskouieDepartment of Basic Sciences, Faculty of Paramedical Sciences, Shahid Beheshti University of Medical Sciences, Tehran, Iran1221ReyhanehFarrokhi YektaProteomics Research Center, Faculty of Paramedical Sciences, Shahid Beheshti University of Medical Sciences, Tehran, Iran1222MostafaRezaie TaviranyProteomics Research Center, Faculty of Paramedical Sciences, Shahid Beheshti University of Medical Sciences, Tehran, Iran1223MasoudSoheili KashaniProteomics Research Center, Faculty of Paramedical Sciences, Shahid Beheshti University of Medical Sciences, Tehran, Iran1224FatemehGoshadrouDepartment of Basic Sciences, Faculty of Paramedical Sciences, Shahid Beheshti University of Medical Sciences, Tehran, Iran1225

en 29849985 Isolation and Proliferation of Spermatogonial Cells from Ghezel Sheep Background: Sheep industry has taken steps toward transforming itself into a more efficient and competitive field. There are many varieties of sheep breeds in the world that each of them serves a useful purpose in the economies of different civilizations. Ghezel sheep is one of the Iranian important breeds that are raised for meat, milk and wool. Field of spermatogonial cell technologies provides tools for genetic improvement of sheep herd and multiple opportunities for research. Spermatogonial cells are the only stem cells capable of transmitting genetic information to future generations.  Methods: This study was designed to extend the technique of isolation and in vitro proliferation of spermatogonial cells in Ghezel sheep.  Results: Isolated cells were characterized further by using specific markers for type A spermatogonia, including PLZF. Also, sertoli cells were characterized by vimentin which is a specific marker for sertoli cells. After 10 days of co-culture, viability rates of the cells was above 94.7%, but after the freezing process the viability rates were 74 percent. Conclusion: In this study, a standard method for isolation and in vitro proliferation of spermatogonial stem cells in Ghezel sheep was developed. Ghezel sheep, Isolation, Spermatogonia 93 97 https://www.ajmb.org/En/Article.aspx?id=308 https://www.ajmb.org/PDF/En/FullText/308.pdf BabakQasemi-PanahiDepartment of Animal Science, Faculty of Agriculture, University of Tabriz, Tabriz, Iran253MansourehMovahedinDepartment of Anatomy, Faculty of Medical Science, University of Tarbiat Modares, Tehran, Iran255GholamaliMoghaddamDepartment of Animal Science, Faculty of Agriculture, University of Tabriz, Tabriz, Iran256ParvizTajikDepartment of Theriogenology, Faculty of Veterinary Medicine, University of Tehran, Tehran, Iran254MortazaKorujiDepartment of Anatomy, Faculty of Medical Science, Iran University of Medical Sciences, Tehran, Iran1226JavadAshrafi-HelanDepartment of Pathobiology, Faculty of Veterinary Medicine, University of Tabriz, Tabriz, Iran1227Seyed AbbasRafatDepartment of Animal Science, Faculty of Agriculture, University of Tabriz, Tabriz, Iran1228

en 29849986 Clinically Significant Dysregulation of hsa-miR-30d-5p and hsa-let-7b Expression in Patients with Surgically Resected Non-Small Cell Lung Cancer Background: The cyclin E2 (CYCE2) is an important regulator in the progression and development of NSCLC, and its ectopic expression promoted the proliferation, invasion, and migration in several tumors, including Non-Small Cell Lung Cancer (NSCLC). However, the upregulation of CYCE2 in NSCLC cells suggested that it has a key role in tumorigenicity. In addition, the RAS family proteins as oncoproteins were activated in many major tumor types and its suitability as the therapeutic target in NSCLC was proposed. Considering the crucial role of microRNAs, it was hypothesized that altered expression of hsa-miR-30d-5p and hsa-let-7b might provide a reliable diagnostic tumor marker for diagnosis of NSCLC. Method: Real-time RT-PCR approach could evaluate the expression alteration of hsa-miR-30d-5p and hsa-let-7b and it was related to the surgically resected tissue of 24 lung cancer patients and 10 non-cancerous patients. The miRNAs expression was associated with clinicopathological features of the patients. Results: Hsa-miR-30d showed a significant downregulation (p=0.0382) in resected tissue of NSCLC patients compared with control group. Its expression level could differentiate different stages of malignancies from each other. The ROC curve analysis gave it an AUC=0.73 (p=0.037) which was a good score as a reliable biomarker. In contrast, hsa-let-7b was significantly overexpressed in tumor samples (p=0.03). Interestingly, our findings revealed a significant association of hsa-let-7b in adenocarcinoma tumors, compared to Squamous Cell Carcinomas (SCC) (p<0.05). Also, analysis of ROC curve of hsa-let-7b (AUC=0.74, p-value=0.042) suggests that it could be as a suitable biomarker for NSCLC. Conclusion: Together, these results suggest a possible tumor suppressor role for hsa-miR-30d in lung tumor progression and initiation. Moreover, upregulation of hsa-let-7b was associated with the tumor type. Lung cancer, MicroRNAs, Tumor markers 98 104 https://www.ajmb.org/En/Article.aspx?id=311 https://www.ajmb.org/PDF/En/FullText/311.pdf Sayed MostafaHosseiniDepartment of Genetics, Faculty of Biological Sciences, Tarbiat Modares University, Tehran, Iran1242BahramMohammad SoltaniDepartment of Genetics, Faculty of Biological Sciences, Tarbiat Modares University, Tehran, Iran1141MahmoudTavallaeiHuman Genetic Research Center, Baqiyatallah University of Medical Sciences, Tehran, Iran1243Seyed JavadMowlaDepartment of Genetics, Faculty of Biological Sciences, Tarbiat Modares University, Tehran, Iran248ElhamTafsiriDepartment of Molecular Medicine, Biotechnology Research Center, Pasteur Institute of Iran, Tehran, Iran1244AbouzarBagheriDepartment of Clinical Biochemistry and Genetics, Molecular and Cell Biology Research Center, Faculty of Medicine, Mazandaran University of Medical Sciences, Sari, Iran1165Hamid RezaKhorram KhorshidGenetic Research Centre, University of Social Welfare and Rehabilitation Sciences, Tehran, Iran42

en 29849987 Tumor Necrosis Factor-Alpha and Interleukin-6 Gene Polymorphisms in Iranian Patients with Ischemic Heart Failure Background: Proinflammatory cytokines have been known to be elevated in patients with Chronic Heart Failure (CHF). Given the importance of proinflammatory cytokines in the context of the failing heart, the prevalence of Tumor Necrosis Factor-α (TNF-α), Interleukin (IL)-6 polymorphisms in patients with CHF was studied due to ischemic heart disease. Methods: Forty three patients with ischemic heart failure were enrolled in this study and compared with 140 healthy individuals. The allele and genotype frequency of four Single Nucleotide Polymorphisms (SNPs) within the IL-6 (-174, nt565) and TNF-α (-308, -238) genes were determined, using Polymerase Chain Reaction with Sequence-Specific Primers (PCR-SSP) assay. Results: The frequency of the TNF-α (-238) A/A genotype was significantly higher in patients comparing to controls (p=0.043), while TNF-α G/A genotype at the same position decreased significantly, in comparison with controls (p=0.018). The most frequent haplotype for TNF-α was A/A in the patient group in comparison with controls (p=0.003). There was no significant difference in allele and genotype frequencies of IL-6 at positions -174 and nt565, and TNF-α at position -308. Conclusion: Certain alleles, genotypes, and haplotypes in TNF-α, but not IL-6, gene were overrepresented in patients with ischemic heart failure, which may, in turn, predispose individuals to this disease. Genes, Heart failure, Interleukin-6, Tumor necrosis factor-alpha 105 109 https://www.ajmb.org/En/Article.aspx?id=309 https://www.ajmb.org/PDF/En/FullText/309.pdf MonaHedayatNetwork of Immunity in Infection, Malignancy and Autoimmunity (NIIMA), Universal Scientific Education and Research Network (USERN), Boston, MA, USA1229Mohammad JafarMahmoudiDivision of Cardiology, Department of Internal Medicine, School of Medicine, Tehran University of Medical Sciences, Tehran, Iran1230MohammadTaghvaeiMolecular Immunology Research Center, Tehran University of Medical Sciences, Tehran, Iran1231EbrahimNematipourTehran Heart Center, Tehran University of Medical Sciences, Tehran, Iran1232ElhamFarhadiHematology Department, Faculty of Allied Medical Science, Iran University of Medical Sciences, Tehran, Iran1057NilufarEsfahanianMolecular Immunology Research Center, Tehran University of Medical Sciences, Tehran, Iran1233MaryamMahmoudiDietitian and Nutrition Experts Team (DiNET), Universal Scientific Education and Research Network (USERN), Tehran, Iran1234MaryamSadrMolecular Immunology Research Center, Tehran University of Medical Sciences, Tehran, Iran1235KeramatNourijelyaniDepartment of Epidemiology and Biostatistics, School of Public Health, Tehran University of Medical Sciences, Tehran, Iran1236Ali AkbarAmirzargarMolecular Immunology Research Center, Tehran University of Medical Sciences, Tehran, Iran179NimaRezaeiMedical Genetics Network (MeGeNe), Universal Scientific Education and Research Network (USERN), Tehran, Iran186

en 29849988 Association of AIRE Polymorphism and the Susceptibility to Multiple Sclerosis in Iranian Population Background: Multiple Sclerosis (MS) is the most common cause of neurologic disability in young adults. Recently, the AIRE gene was identified as a genetic risk factor for several autoimmune diseases in genome wide association studies. The aim of this study was to further investigate the possible role of the AIRE gene in susceptibility to MS in Iranian population. Methods: A total of 112 MS patients and 94 ethnically matched controls were included in the study. The Single-Nucleotide Polymorphism (SNP) (rs1800520, C>G) with a global MAF=0.2282/1143 was selected and genotyped using HRM real-time PCR method. Results: Results showed that AIRE SNP rs1800520 was significantly less common in the MS patients than in healthy controls (17.8 vs. 28.7%, pc=0.032, OR=0.54,95% CI 0.279,1.042). Also, the frequency of allele G was significantly higher among the control group than in the case group (37.77 vs. 25%, pc=0.014). Interestingly, mRNA transcribed on the rs1800520 SNP showed decreased free energy than the wild type suggesting that its increased stability may be responsible for the different activities of the polymorphic AIRE molecule.  Conclusions: This is the first study investigating the relationship between AIRE gene and the susceptibility to MS. These results indicated that the rs1800520 SNP is not a susceptibility gene variant for the development of MS in Iranian population. AIRE, Iran, Multiple sclerosis, Single-nucleotide polymorphism 110 114 https://www.ajmb.org/En/Article.aspx?id=310 https://www.ajmb.org/PDF/En/FullText/310.pdf TaherehSadeghian-RiziDepartment of Pharmaceutical Biotechnology, Faculty of Pharmacy, Isfahan University of Medical Sciences, Isfahan, Iran1237FereshtehAlsahebfosoulDepartment of Immunology, Faculty of Medicine, Isfahan University of Medical Sciences, Isfahan, Iran1238MohammadKazemiDepartment of Genetics and Molecular Biology, Faculty of Medicine, Isfahan University of Medical Sciences, Isfahan, Iran1239HosseinKhanahmadDepartment of Genetics and Molecular Biology, Faculty of Medicine, Isfahan University of Medical Sciences, Isfahan, Iran162AliJahanian NajafabadiDepartment of Pharmaceutical Biotechnology, Faculty of Pharmacy, Isfahan University of Medical Sciences, Isfahan, Iran301

en 29849989 Evaluating the Frequency of aac(6')-IIa, ant(2'')-I, intl1, and intl2 Genes in Aminoglycosides Resistant Klebsiella pneumoniae Isolates Obtained from Hospitalized Patients in Yazd, Iran Background: Klebsiella pneumoniae (K. pneumoniae) is an opportunistic pathogen that could be resistant to many antimicrobial agents. Resistance genes can be carried among gram-negative bacteria by integrons. Enzymatic inactivation is the most important mechanism of resistance to aminoglycosides. In this study, the frequencies of two important resistance gene aac(6')-IIa and ant(2'')-I, and genes coding integrase I and II, in K. pneumoniae isolates resistant to aminoglycosides were evaluated. Methods: In this cross-sectional study, an attempt was made to assess the antibiotic susceptibility of 130 K. pneumoniae isolates obtained from different samples of patients hospitalized in training hospitals of Yazd evaluated by disk diffusion method. The frequencies of aac(6')-IIa, ant(2'')-I, intl1, and intl2 genes were determined by PCR method. Data were analyzed by chi-square method using SPSS software (Ver. 16). Results: our results showed that resistance to gentamicin, tobramycin, kanamycin, and amikacin were 34.6, 33.8, 43.8, and 14.6%, respectively. The frequencies of aac(6')-IIa, ant(2'')-I, intl1, and intl2 genes were 44.6, 27.7, 90, and 0%, respectively. Conclusion: This study showed there are high frequencies of genes coding aminoglycosides resistance in K. pneumoniae isolates. Hence, it is very important to monitor and inhibit the spread of antibiotic resistance genes. Aminoglycosides, Drug resistance, Integrons, Klebsiella pneumoniae, Microbial 115 119 https://www.ajmb.org/En/Article.aspx?id=313 https://www.ajmb.org/PDF/En/FullText/313.pdf HesamMokhtariInternational Campus, Shahid Sadoughi University of Medical Sciences, Tehran, Iran1252GildaEslamiDepartment of Parasitology and Mycology, Faculty of Medicine, Shahid Sadoughi University of Medical Sciences, Yazd, Iran1253HengamehZandiDepartment of Microbiology, Faculty of Medicine, Shahid Sadoughi University of Medical Sciences, Yazd, Iran1254AminDehghan-Banadkouki Department of Pathobiology, Faculty of Public Health, Tehran University of Medical Sciences, Tehran, Iran1255MahmoodVakiliDepartment of Public Medicine, Faculty of Medicine, Shahid Sadoughi University of Medical Sciences, Yazd, Iran1256

en 29849990 Assessment of EGFR Gene Expression Following Vitrification of 2-cell and Blastocyst Mouse Embryos Background: Exact mechanisms of fetal harm following vitrification are still unknown. This study was conducted to evaluate the cryopreservation impact on the expression of Epidermal Growth Factor Receptor (EGFR) gene in mouse 2-cell and blastocysts. Methods: To stimulate ovulation in mice, hCG was injected, followed by collecting 2-cells and blastocysts after 44-46 and 88-89 hr, respectively. These embryos were divided into two case and control groups. The fresh case group was cryopreserved using cryotop and warmed after 4 mounts. Normal 2-cells were selected based on their morphology and their RNA was extracted. Quantitative expression of EGFR gene in both groups was investigated by applying real time-PCR. Results: The statistical real-time (RT)-PCR analyses performed using SPSS revealed that the expression level of EGFR gene was diminished in the case group compared to the control group.  Conclusion: The current study indicated the negative effect of cryopreservation on expression amount of EGFR gene in 2-cell and blastocyst mouse embryos. Blastocyst, Cryopreservation, Embryo, Gene expression, Vitrification 120 122 https://www.ajmb.org/En/Article.aspx?id=334 https://www.ajmb.org/PDF/En/FullText/334.pdf RouhollahGazorDepartment of Anatomy and Cell Biology, Faculty of Medicine, Guilan University of Medical Sciences, Rasht, Iran1337MozhganEskandariDepartment of Anatomy, Ardabil University of Medical Sciences, Ardabil, Iran1338AlirezaSharafshahCellular and Molecular Research Center, Faculty of Medicine, Guilan University of Medical Sciences, Rasht, Iran1339Mohammad HadiBahadoriDepartment of Anatomy and Cell Biology, Faculty of Medicine, Guilan University of Medical Sciences, Rasht, Iran1340Mohammad GhasemGolmohammadiDepartment of Anatomy, Ardabil University of Medical Sciences, Rasht, Iran1341ParvanehKeshavarzCellular and Molecular Research Center, Faculty of Medicine, Guilan University of Medical Sciences, Rasht, Iran1342

en 29849219 Retraction: The Frequency and Importance of Common α-globin Gene Deletions Among β-Thalassemia Carriers in an Iranian Population The Editorial Board of Avicenna Journal of Medical Biotechnology (AJMB) has decided to retract the original article entitled “The Frequency and Importance of Common α-globin Gene Deletions Among β-Thalassemia Carriers in an Iranian Population” published in the October-December 2017 issue due to a fact which is contrary to the scientific rules and regulation of AJMB. Retract, Retraction 123 123 https://www.ajmb.org/En/Article.aspx?id=10360 https://www.ajmb.org/PDF/En/FullText/10360.pdf AzamMoosavi1171AliM. Ardekani2