Your search keyword '"Electrophoresis"' showing total 94 results

1. A novel α0‐thalassemia deletion in a Brazilian child with Hb H disease: −−Mococa.

Author

Soler, A. M., Pedroso, G. A., Geraldo, A. P. M., Albuquerque, D. M., Costa, F. F., Santos, M. N. N., Knijnenburg, J., Harteveld, C. L., Sonati, M. F., and da Luz, J. A.

Subjects

*HEMOGLOBINOPATHY genetics, *HYPOCHROMIC anemia, *HIGH performance liquid chromatography, *ALPHA-Thalassemia, *BLOOD collection, *POLYMERASE chain reaction, *HEMOGLOBINOPATHY, *FAMILY history (Medicine), *DNA, *GENETIC carriers, *GENES, *BRAZILIANS, *GENETIC polymorphisms, *GENETIC mutation, *BLOOD diseases, *ELECTROPHORESIS, *SEQUENCE analysis, *RETICULOCYTES, *GENOTYPES, *PHENOTYPES

Published

2024

2. A novel α0‐thalassemia deletion in a Brazilian child with Hb H disease: −−Mococa.

Author

Soler, A. M., Pedroso, G. A., Geraldo, A. P. M., Albuquerque, D. M., Costa, F. F., Santos, M. N. N., Knijnenburg, J., Harteveld, C. L., Sonati, M. F., and da Luz, J. A.

Subjects

HEMOGLOBINOPATHY genetics, HYPOCHROMIC anemia, HIGH performance liquid chromatography, ALPHA-Thalassemia, BLOOD collection, POLYMERASE chain reaction, HEMOGLOBINOPATHY, FAMILY history (Medicine), DNA, GENETIC carriers, GENES, BRAZILIANS, GENETIC polymorphisms, GENETIC mutation, BLOOD diseases, ELECTROPHORESIS, SEQUENCE analysis, RETICULOCYTES, GENOTYPES, PHENOTYPES

Published

2024

3. Spa typing of Methicillin-Resistant Staphylococcus aureus isolated from clinical samples of hospitalized patients, a study in the Wasit province of Iraq.

Author

Alhakeem, Karar, Nemati, Mostafa, Pourahmad, Fazel, and Alshimry, Hussam Sami

Subjects

DNA analysis, BACTERIAL protein analysis, CHLORAMPHENICOL, STAPHYLOCOCCAL diseases, RESEARCH funding, MICROBIAL sensitivity tests, TETRACYCLINE, DRUG resistance in microorganisms, HOSPITAL care, POLYMERASE chain reaction, AGAR, METHICILLIN-resistant staphylococcus aureus, VANCOMYCIN resistance, DISEASE prevalence, CLINDAMYCIN, GENTAMICIN, ERYTHROMYCIN, IMIPENEM, STAINS & staining (Microscopy), ELECTROPHORESIS, SEQUENCE analysis, PENICILLIN, CEFOXITIN, RIFAMPIN, HOSPITAL wards

Abstract

Introduction: Since its discovery in 1961, methicillin-resistant Staphylococcus aureus (MRSA) has been recognized as a significant healthcare-associated pathogen (HA-MRSA) and a notorious 'superbug'. Typing is crucial for surveillance, epidemiology analysis, infection control of MRSA and sequencing of the spa gene is one of the most common methods used for determining the origin of this bacterium in humans and animals. This research aimed to determine the antibiotic resistance and spa type of S. aureus strains collected from outpatients in two hospitals in the Wasit province of Iraq. Material & Methods: The study analyzed 200 outpatient MRSA isolates by collecting nasal and sputum samples from patients. Standard biochemical and molecular methods based on the nuc gene were used to identify S. aureus bacteria and amplify the mecA and spa genes. The Kirby-Bauer disc diffusion method was employed to determine the antibiotic sensitivity of the isolates using penicillin, cefoxitin, vancomycin, gentamicin, erythromycin, tetracycline, imipenem, clindamycin, chloramphenicol and rifampicin. Results: Methods. The prevalence of MRSA was more common in women than in men. Antibiogram results showed that most of the isolates were resistant to penicillin (94.2%) and sensitive to imipenem (100%), clindamycin (100%), and chloramphenicol (100%). Of these 35 isolates, 30 (87.5%) and 26 strains (74.3%) were positive for the mecA and spa genes. Typing based on spa gene sequencing revealed four different patterns: t386, t3579, U0002 and U0234. Conclusion: Variations in the spa gene among different S. aureus isolates may he of clinical importance when treating staphylococcal infections. In this study, spa typing revealed four different patterns in Iraq, representing diagnostic and therapeutic implications. [ABSTRACT FROM AUTHOR]

Published

2024

4. Next-generation sequencing in laboratory medicine.

Author

Chandra, Rajasri

Subjects

*RNA analysis, *DNA analysis, *GENOME-wide association studies, *POLYMERASE chain reaction, *GENE expression, *PATHOLOGICAL laboratories, *ELECTROPHORESIS, *SEQUENCE analysis

Abstract

The article focuses on the impact of next-generation sequencing (NGS) technology in laboratory medicine, which has revolutionized disease diagnosis, prognosis, therapeutic decisions, and patient follow-up. It discusses the limitations of Sanger sequencing, which led to the development of NGS technologies capable of sequencing large numbers of DNA sequences simultaneously, offering faster and less expensive options for clinical applications.

Published

2024

5. Familial chylomicronemia syndrome: case reports of siblings with deletions of the GPIHBP1 gene.

Author

Kim, Ka Young, Heo, You Joung, Ko, Jung Min, Lee, Young Ah, Shin, Choong Ho, Ki, Chang Seok, and Lee, Yun Jeong

Subjects

*HDL cholesterol, *HYPERCHOLESTEREMIA, *HYPERLIPOPROTEINEMIA, *AUTOANTIBODIES, *POLYMERASE chain reaction, *GENE expression, *PANCREATITIS, *LIPASES, *TRIGLYCERIDES, *GENETIC mutation, *ELECTROPHORESIS, *GENETIC testing, *SEQUENCE analysis

Abstract

Background: Familial chylomicronemia syndrome (FCS) is a rare monogenic form of severe hypertriglyceridemia, caused by mutations in genes involved in triglyceride metabolism. Herein, we report the case of a Korean family with familial chylomicronemia syndrome caused by compound heterozygous deletions of glycosylphosphatidylinositol-anchored high-density lipoprotein-binding protein 1 (GPIHBP1). Case presentation: A 4-year-old boy was referred for the evaluation of severe hypertriglyceridemia (3734 mg/dL) that was incidentally detected 4 months prior. His elder brother also demonstrated an elevated triglyceride level of 2133 mg/dL at the age of 9. Lipoprotein electrophoresis revealed the presence of chylomicrons, an increase in the proportion of pre-beta lipoproteins, and low serum lipoprotein lipase levels. The patient's parents and first elder brother had stable lipid profiles. For suspected FCS, genetic testing was performed using the next-generation sequencing-based analysis of 31 lipid metabolism-associated genes, which revealed no pathogenic variants. However, copy number variant screening using sequencing depth information suggested large heterozygous deletion encompassing all the coding exons of GPIHBP1. A real-time quantitative polymerase chain reaction was performed to validate the deletion site. The results showed that the siblings had two heterozygous copy number variants consisting of the whole gene and an exon 4 deletion, each inherited from their parents. During the follow-up period of 17 months, the patient did not develop pancreatitis, following dietary intervention. Conclusion: These siblings' case of familial chylomicronemia syndrome caused by rare GPIHBP1 deletions highlight the implementation of copy number variants—beyond next-generation sequencing—as an important consideration in diagnosis. Accurate genetic diagnosis is necessary to establish the etiology of severe hypertriglyceridemia, which increases the risk of pancreatitis. [ABSTRACT FROM AUTHOR]

Published

2024

6. Molecular diagnosis of hereditary hemolytic anemias: Recent updates.

Author

Agarwal, Archana M. and Rets, Anton V.

Subjects

*GENETIC disorder diagnosis, *HEMOLYTIC anemia, *MOLECULAR diagnosis, *SEQUENCE analysis, *PAPER chromatography, *CELL membranes, *ELECTROPHORESIS, *ERYTHROPOIESIS, *ERYTHROCYTES, *POLYMERASE chain reaction

Abstract

Hereditary hemolytic anemia (HHA) is a heterogeneous group of disorders due to genetically caused defects in red blood cell membrane structure, enzymes, heme and globin synthesis, erythroid proliferation, and differentiation. Traditionally, the diagnostic process is complex and includes a plethora of tests from routine to highly specialized ones. The inclusion of molecular testing has significantly improved the diagnostic yield. The value of molecular testing is broader than just rendering the correct diagnosis, as it may also guide therapeutic decisions. As more molecular modalities become available for clinical use, it is imperative to understand their benefits and disadvantages pertaining to the HHA diagnostics. Re‐evaluation of the traditional diagnostic workflow may also bring forth additional benefits. This review focuses on the current state of molecular testing for HHA. [ABSTRACT FROM AUTHOR]

Published

2023

7. A novel stop codon mutation in STK11 gene is associated with Peutz-Jeghers Syndrome and elevated cancer risk: a case study.

Author

Khanabadi, Binazir, Seyfi, Diba Najafgholizadeh, Rejali, Leili, Taleghani, Mohammad Yaghoob, Tavallaei, Mehdi, Shahrokh, Shabnam, Abkenar, Elahe Daskar, Noukabadi, Fatemeh Naderi, Aghdaei, Hamid Asadzadeh, and Mojarad, Ehsan Nazemalhosseini

Subjects

*BIOMARKERS, *STOMACH, *GENETIC mutation, *SEQUENCE analysis, *COLONOSCOPY, *COLON (Anatomy), *STAINS & staining (Microscopy), *INTESTINAL polyps, *ELECTROPHORESIS, *BLOOD collection, *COLORECTAL cancer, *TRYPTOPHAN, *TUMOR suppressor genes, *HAMARTOMA, *AGAR, *PEUTZ-Jeghers syndrome, *ABDOMINAL pain, *COMPUTED tomography, *ENDOSCOPIC gastrointestinal surgery, *POLYMERASE chain reaction, *TYROSINE, *FAMILY history (Medicine), *DISEASE risk factors

Abstract

Based on the analysis of patients with Peutz-Jeghers syndrome (PJS), Serine threonine kinase11 (STK11) is known as a tumor suppressor gene, which is involved in cell polarization, regulation of apoptosis, and DNA damage response. In this case report study, we examined STK11 gene sequencing in a 42-year-old woman with mucocuta neous pigmentation and positive family history. Endoscopy and colonoscopy showed >1000 polyps throughout the stomach/colon (PJ-type hamartomas). The larger polyp in the stomach was resected and the small bowel imaging detected multiple jejunum/ileum small polyps. The data released from the sequencing results revealed five alterations in exons 1 to 5. The major mutation in stop codon was reported as converted to the amino acid tryptophan (TRP) to tyrosine (TER). The TGG codon was converted to TAG by mutation. Finally, another novel mutation in STK11 stop codon as a 'de novo' variant was seen. It is predicted that stop codon mutations make the affected person susceptible to developing colorectal cancer. [ABSTRACT FROM AUTHOR]

Published

2023

8. Ginseng-Containing Sijunzi Decoction Ameliorates Ulcerative Colitis by Orchestrating Gut Homeostasis in Microbial Modulation and Intestinal Barrier Integrity.

Author

Wu, Yuqi, Zheng, Yanfei, Wang, Xiaolu, Tang, Ping, Guo, Wenqian, Ma, Han, Zhang, Anqi, Li, Delong, Xie, Yuxin, Wang, Chong-Zhi, Yao, Haiqiang, Wan, Jin-Yi, and Yuan, Chun-Su

Subjects

*ULCERATIVE colitis, *HOMEOSTASIS, *CYTOKINES, *INTERLEUKINS, *HERBAL medicine, *SEQUENCE analysis, *SPECTROPHOTOMETERS, *HIGH performance liquid chromatography, *GUT microbiome, *ANTI-inflammatory agents, *ANIMAL experimentation, *WESTERN immunoblotting, *ELECTROPHORESIS, *ONE-way analysis of variance, *INTERFERONS, *T-test (Statistics), *COMPARATIVE studies, *RESEARCH funding, *TUMOR necrosis factors, *ENZYME-linked immunosorbent assay, *AGAR, *DESCRIPTIVE statistics, *MASS spectrometry, *GLYCOPROTEINS, *BILE acids, *INTESTINAL mucosa, *FECAL microbiota transplantation, *DATA analysis software, *POLYMERASE chain reaction, *EPITHELIAL cells, *GINSENG, *CHINESE medicine, *MICE, *DISEASE remission, *ESCHERICHIA, *PHARMACODYNAMICS, *DRUG administration, *DRUG dosage

Abstract

Ulcerative colitis (UC) has become a global epidemic, and the lack of an effective cure highlights the necessity and urgency to explore novel therapies. Sijunzi Decoction (SJZD), a classical Chinese herbal formula, has been comprehensively applied and clinically proven effective in treating UC; however, the pharmacological mechanism behind its therapeutic benefits is largely obscure. Here, we find that SJZD can restore microbiota homeostasis and intestinal barrier integrity in DSS-induced colitis. SJZD significantly alleviated the colonic tissue damage and improved the goblet cell count, MUC2 secretion, and tight junction protein expressions, which indicated enhanced intestinal barrier integrity. SJZD remarkedly suppressed the abundance of phylum Proteobacteria and genus Escherichia-Shigella, which are typical features of microbial dysbiosis. Escherichia-Shigella was negatively correlated with body weight and colon length, and positively correlated with disease activity index and IL-1 β. Furthermore, through gut microbiota depletion, we confirmed that SJZD exerted anti-inflammatory activities in a gut microbiota-dependent manner, and fecal microbiota transplantation (FMT) validated the mediating role of gut microbiota in the SJZD treatment of UC. Through gut microbiota, SJZD modulates the biosynthesis of bile acids (BAs), especially tauroursodeoxycholic acid (TUDCA), which has been identified as the signature BA during SJZD treatment. Cumulatively, our findings disclose that SJZD attenuates UC via orchestrating gut homeostasis in microbial modulation and intestinal barrier integrity, thus offering a promising alternative approach to the clinical management of UC. [ABSTRACT FROM AUTHOR]

Published

2023

9. Assessment of Bacterial Diversity of Industrial Poultry Wastewater by Denaturing Gradient Gel Electrophoresis (DGGE) and the Cultivation Method in Order to Inform Its Reuse in Agriculture.

Author

Oueslati, Amira, Hassen, Wafa, Ellafi, Ali, Alibi, Sana, Jaziri, Ahlem, Bachkouel, Sarra, Oueslati, Imen, Snoussi, Mejdi, Adnan, Mohd, Patel, Mitesh, Elasbali, Abdelbaset Mohamed, and Mansour, Hedi Ben

Subjects

*BIOCHEMISTRY, *POULTRY, *DNA, *SEQUENCE analysis, *AGRICULTURE, *ELECTROPHORESIS, *PHENOMENOLOGICAL biology, *VIRAL load, *RNA, *AQUATIC microbiology, *GENOMES, *DESCRIPTIVE statistics, *SEWAGE, *POLYMERASE chain reaction

Abstract

Effluents discharged by poultry meat industries are heavily polluted with raw materials, such as fat, blood residues, and proteins. Thus, untreated effluents directly discharged into the environment may constitute a public health threat. This study aims to evaluate the bacterial diversity of three water qualities: industrial poultry wastewater (PWW), tap water (TW), and PWW diluted with TW (50 : 50) (V/V) (TWPWW) by the combination of culture-independent and culture-dependent approaches. The total bacterial DNA was extracted using phenol/chloroform method. The hypervariable 16S rRNA region V3-V5 was amplified by PCR using universal primers. The amplicons were separated by vertical electrophoresis on a polyacrylamide gel of increasing denaturing gradient according to their richness in GC bases. Selected bands were reamplified and sequenced. Pure isolated bacteria from nutrient agar medium were characterized according to their morphological and biochemical characteristics. Genomic DNA from pure strains was extracted by boiling method, and a molecular amplification of the 16S–23S ITS region of the 16S rRNA gene was performed using the universal primers. Selected isolates were identified by sequencing. Results showed a high bacterial load and diversity in PWW in comparison with TW and TWPWW. A collection of 44 strains was obtained, and 25 of them were identified by sequencing. Proteobacteria represented 76% of isolated bacteria Gamma-Proteobacteria was the predominate isolate (68%). Other isolates were Firmicutes (8%), Bacteroidetes (12%), and Actinobacteria (8%). These isolates belong to different genera, namely, Pseudomonas, Acinetobacter, Proteus, Empedobacter, Corynebacterium, Enterobacter, Comamonas, Frondibacter, Leclercia, Staphylococcus, Atlantibacter, Klebsiella, and Microbacterium. [ABSTRACT FROM AUTHOR]

Published

2022

10. Comprehensive Evaluation of Serum tRF-17-WS7K092 as a Promising Biomarker for the Diagnosis of Gastric Cancer.

Author

Gu, Xinliang, Zhang, Yu, Huang, Yuejiao, and Ju, Shaoqing

Subjects

*STOMACH tumors, *TRANSFER RNA, *SEQUENCE analysis, *ELECTROPHORESIS, *LYMPH nodes, *METASTASIS, *GENE expression, *DNA-binding proteins, *AGAR, *TUMOR markers, *POLYMERASE chain reaction, *RECEIVER operating characteristic curves, *SENSITIVITY & specificity (Statistics), *SYMPTOMS

Abstract

Background. Gastric cancer (GC) is a malignant tumor of the gastrointestinal system. Since the early symptoms of GC are not obvious and lack efficient diagnostic markers, it is urgent to find new diagnostic markers with good sensitivity and specificity. tRNA-derived small RNAs (tsRNAs) are an emerging class of small noncoding RNAs with good abundance in body fluids. We aim to find new tsRNAs as biomarkers for GC diagnosis. Methods. High-throughput sequencing was used to identify differentially expressed tsRNAs in GC tissues, and quantitative real-time PCR was used to detect the expression level of tRF-17-WS7K092. Agarose gel electrophoresis and Sanger sequencing were performed to verify the characteristics of tRF-17-WS7K092. The diagnostic efficacy of tRF-17-WS7K092 was analyzed by the receiver operating characteristic curve. Results. In this study, the expression levels of tRF-17-WS7K092 were significantly increased in GC tissues, cells, and serum. After GC surgery, the expression level of serum tRF-17-WS7K092 decreased, and its high expression was associated with low survival rates. In addition, the expression level of serum tRF-17-WS7K092 was correlated with the T stage, TNM stage, lymph node metastasis, and nerve/vascular invasion and could distinguish GC patients from gastritis patients and healthy donors as well. Conclusions. The expression of serum tRF-17-WS7K092 was significantly increased in GC and decreased after GC surgery, suggesting that serum tRF-17-WS7K092 may serve as a promising biomarker for the diagnostic and prognostic monitoring of GC. [ABSTRACT FROM AUTHOR]

Published

2022

11. Immunosuppressive Activity of Campylobacter Jejuni Isolates in Relation to the Cellular Link of the Body's Immunoprotection.

Author

Mazur, Tetiana, Shchur, Nataliia, and Boianovskyi, Serhii

Subjects

*SEQUENCE analysis, *ELECTROPHORESIS, *CULTURE media (Biology), *CAMPYLOBACTER infections, *IMMUNOSUPPRESSION, *NUCLEOTIDES, *CAMPYLOBACTER, *FOOD poisoning, *GENES, *GENOMES, *DESCRIPTIVE statistics, *POLYMERASE chain reaction, *TOXINS, *NUCLEIC acid amplification techniques

Abstract

Global environmental changes have caused transformations in the biology of microorganisms, especially among campylobacter, which are currently associated with food toxic infections. The means of influence of these bacteria on susceptible organisms, namely toxins, have not been finally clarified. The purpose of this study was to investigate the genetic conditionality of toxin formation in isolates of Campylobacter jejuni and determination of the degree of inhibition of the body's protective reactions by toxic fractions of Campylobacter protein compounds. The methodology of this study was based on the polymerase chain reaction using primers to indicate the nucleotide sequences of the Campylobacter jejuni genome that encode the synthesis of toxins. Samples from 4 Campylobacter isolates were examined for the content of protein fractions according to the Lowry assay. The analysis of the electropherogram of the results of DNA amplification in a comparative aspect with the data of standard samples allowed establishing the presence of genome elements that indicate the potential ability to produce toxins in Campylobacter jejuni isolates sampled from the material under study. Toxic fractions separated from the supernatant of Campylobacter jejuni broth culture are represented by protein-carbohydrate substances. The obtained peak toxigenic fractions of the dialysate of the bacterial culture sediment contained protein within 9.5-17 μg/ml. In the dialysate of the broth culture supernatant, where 5 groups of toxigenic fractions were distinguished, their protein content ranged within 10-85 μg/ml. By reproducing the opsono-phagocytic reaction involving toxigenic fractions of Campylobacter jejuni, a sufficiently pronounced immunosuppressive effect of these complexes on the body of warm-blooded animals was established with an opsonic index of 2.6 ± 0.03. The obtained results allow clarifying the connection between toxin formation in Campylobacter jejuni and their immunosuppressive effect on the body of warm-blooded animals and humans, which in the future will positively affect the improvement of measures for the prevention and treatment of animals with this pathology [ABSTRACT FROM AUTHOR]

Published

2022

12. Analysis of circRNAs profile in TNF-α treated DPSC.

Author

Lei, Qiyin, Liang, Zezi, Lei, Qiaoling, Liang, Fuying, Ma, Jing, Wang, Zhongdong, and He, Shoudi

Subjects

CIRCULAR RNA, DENTAL pulp diseases, SEQUENCE analysis, INFLAMMATION, ELECTROPHORESIS, DENTAL pulp, BIOINFORMATICS, GENE expression, CELLULAR signal transduction, TUMOR necrosis factors, STEM cells, CELL proliferation, AGAR, MESSENGER RNA, MITOGEN-activated protein kinases, POLYMERASE chain reaction

Abstract

Background: Pulpitis often are characterized as sustained inflammation and impaired pulp self-repair. Circular RNAs (circRNAs) have been reported to be involved in the development of inflammation, but their influence in pulpitis is still unidentified, which was examined in our research. Methods: In this study, TNF-α (20 ng/mL) was used to treat DPSCs, then MTS identified cell proliferation. The circRNAs profile in DPSCs with or without TNF-α treatment was evaluated using RNA sequencing and subsequently by bioinformatics analysis. After that, the circular structure was assessed using agarose gel electrophoresis, followed by Sanger sequencing. And the circRNAs expression was ratified using quantitative real-time polymerase chain reaction in cell and tissues samples. Additionally, the plausible mechanism of circRNAs was envisaged, and the circRNA-miRNA-mRNA linkage was plotted using Cytoscape. Results: The treatment of TNF-α inhibited cell proliferation capabilities in DPSCs, which also made 1195 circRNA expressions undergo significant alterations. Among these changes, 11 circRNAs associated with inflammation were chosen for circular structure verification, and only seven circRNAs (hsa_circ_0001658, hsa_circ_0001978, hsa_circ_0003910, hsa_circ_0004314, hsa_circ_0004417, hsa_circ_0035915, and hsa_circ_0002545) had circular structure. Additionally, five circRNAs expressions (hsa_circ_0001978, hsa_circ_0003910, hsa_circ_0004314, hsa_circ_0004417, and hsa_circ_0035915) had significantly altered between with or without TNF-α treated DPSCs. Furthermore, hsa_circ_0001978 and hsa_circ_0004417 were increased in patients suffering from pulpitis. Furthermore, their ceRNA linkage and Kyoto Encyclopedia of Genes and Genomes analysis suggested that these two circRNAs may participate in the inflammation development of pulpitis via mitogen-activated protein kinase and the Wnt signaling pathway. Conclusion: This study revealed that the circRNAs profile was altered in TNF-α treated DPSCs. Also, hsa_circ_0001978 and hsa_circ_0004417 may be involved in the inflammation progress of pulpitis. These outcomes provided the latest information for additional research on pulpitis. [ABSTRACT FROM AUTHOR]

Published

2022

13. Molecular epidemiology and characterization of multiple drug-resistant (MDR) clinical isolates of Acinetobacter baumannii

Author

El-Shazly, Sherief, Dashti, Ali, Vali, Leila, Bolaris, Michael, and Ibrahim, Ashraf S

Subjects

Medical Microbiology, Biomedical and Clinical Sciences, Clinical Sciences, Infectious Diseases, Prevention, Vaccine Related, Antimicrobial Resistance, Biotechnology, Genetics, Infection, Acinetobacter Infections, Acinetobacter baumannii, DNA Transposable Elements, DNA, Bacterial, Drug Resistance, Multiple, Bacterial, Electrophoresis, Gel, Pulsed-Field, Gene Expression Regulation, Bacterial, Genotype, Hospitals, Humans, Los Angeles, Molecular Epidemiology, Multilocus Sequence Typing, Polymerase Chain Reaction, Sequence Analysis, DNA, beta-lactamase, MLST, PFGE, β-lactamase, Microbiology, Public Health and Health Services, Clinical sciences, Epidemiology, Public health

Abstract

ObjectivesThe aim of this study was to identify the genetic relatedness of multiple drug-resistant (MDR) Acinetobacter baumannii clinical isolates recovered from a hospital in Los Angeles.MethodsTwenty-one MDR A. baumannii isolates were collected and their antibiotic susceptibilities determined according to Clinical and Laboratory Standards Institute guidelines. Genes coding for antibiotic resistance were identified by PCR, and their identities were confirmed by DNA sequencing. Clonal relationships were studied by pulsed-field gel electrophoresis (PFGE) and multilocus sequence typing (MLST).ResultsMDR consistently correlated with the presence of oxacillinases, mostly in the form of the plasmid-mediated OXA-23 enzyme, which was detected in 12 (57.1%) isolates. GES-type carbapenemases were found in 20 (95.2%) strains, AAC in all 21 (100%) strains, and PER in seven (33.3%) strains, and ISAba1 was detected in 16 (76.2%) isolates. The association between ISAba1 and resistance genes confirms insertion elements as a source of β-lactamase production. Of the 21 clinical isolates, five were found to be related to sequence type 1 (ST1) and 16 to ST2, as analyzed by MLST. PFGE demonstrated that the majority of clinical isolates were highly related (>85%).ConclusionsThis study supports a more complete understanding of genotyping of antibiotic resistance for better assessment of MDR strain transmission.

Published

2015

14. Variants on the UBE2L3/YDJC Autoimmune Disease Risk Haplotype Increase UBE2L3 Expression by Modulating CCCTC‐Binding Factor and YY1 Binding.

Author

Gopalakrishnan, Jaanam, Tessneer, Kandice L., Fu, Yao, Pasula, Satish, Pelikan, Richard C., Kelly, Jennifer A., Wiley, Graham B., and Gaffney, Patrick M.

Subjects

*PROTEINS, *CHROMOSOMES, *GENETIC mutation, *SEQUENCE analysis, *GENETICS, *ELECTROPHORESIS, *NUCLEAR proteins, *GENETIC variation, *AUTOIMMUNE diseases, *SIGNAL peptides, *ALLELES, *QUANTITATIVE research, *PRECIPITIN tests, *RNA, *GENE expression, *CELLULAR signal transduction, *BIOINFORMATICS, *HAPLOTYPES, *ENZYMES, *EPSTEIN-Barr virus, *DISEASE susceptibility, *BIOLOGICAL assay, *OXIDOREDUCTASES, *SEX chromatin, *POLYMERASE chain reaction, *MEMBRANE proteins, *TRANSCRIPTION factors, *CARRIER proteins

Abstract

Objective: Genetic variants spanning UBE2L3 are associated with increased expression of the UBE2L3‐encoded E2 ubiquitin‐conjugating enzyme H7 (UbcH7), which facilitates activation of proinflammatory NF‐κB signaling and susceptibility to autoimmune diseases. We undertook this study to delineate how genetic variants carried on the UBE2L3/YDJC autoimmune risk haplotype function to drive hypermorphic UBE2L3 expression. Methods: We used bioinformatic analyses, electrophoretic mobility shift assays, and luciferase reporter assays to identify and functionally characterize allele‐specific effects of risk variants positioned in chromatin accessible regions of immune cells. Chromatin conformation capture with quantitative polymerase chain reaction (3C‐qPCR), chromatin immunoprecipitation (ChIP)–qPCR, and small interfering RNA (siRNA) knockdown assays were performed on patient‐derived Epstein‐Barr virus–transformed B cells homozygous for the UBE2L3/YDJC nonrisk or risk haplotype to determine if the risk haplotype increases UBE2L3 expression by altering the regulatory chromatin architecture in the region. Results: Of the 7 prioritized variants, 5 demonstrated allele‐specific increases in nuclear protein binding affinity and regulatory activity. High‐throughput sequencing of chromosome conformation capture coupled with ChIP (HiChIP) and 3C‐qPCR uncovered a long‐range interaction between the UBE2L3 promoter (rs140490, rs140491, rs11089620) and the downstream YDJC promoter (rs3747093) that was strengthened in the presence of the UBE2L3/YDJC risk haplotype, and correlated with the loss of CCCTC‐binding factor (CTCF) and gain of YY1 binding at the risk alleles. Depleting YY1 by siRNA disrupted the long‐range interaction between the 2 promoters and reduced UBE2L3 expression. Conclusion: The UBE2L3/YDJC autoimmune risk haplotype increases UBE2L3 expression through strengthening a YY1‐mediated interaction between the UBE2L3 and YDJC promoters. [ABSTRACT FROM AUTHOR]

Published

2022

15. Conformation sensitive gel electrophoresis for the detection of calreticulin mutations in BCR‐ABL1‐negative myeloproliferative neoplasms.

Author

Zakaria, Nur Atikah, Rosle, Norfifiana Alisa, Siti Asmaa, Mat Jusoh, Aziee, Sudin, Haiyuni, Mohd Yassim, Samat, Nurul Ameera, Husin, Azlan, Hassan, Rosline, Ramli, Marini, Mohamed Yusoff, Shafini, Ibrahim, Ibrahim Khidir, Al‐Jamal, Hamid Ali Nagi, and Johan, Muhammad Farid

Subjects

*DISEASE clusters, *GENETIC mutation, *SEQUENCE analysis, *CONFIDENCE intervals, *ELECTROPHORESIS, *MYELOPROLIFERATIVE neoplasms, *CANCER patients, *AGAR, *HEMATOLOGIC malignancies, *DESCRIPTIVE statistics, *CALCIUM-binding proteins, *POLYMERASE chain reaction, *MOLECULAR structure, *ODDS ratio

Abstract

Introduction: Calreticulin (CALR) mutations in myeloproliferative neoplasms (MPN) have been reported to be key markers in the molecular diagnosis, particularly in patients lacking JAK2 V617F mutation. In most current reports, CALR mutations were analysed by either allele‐specific PCR (AS‐PCR), or the more expensive quantitative real‐time PCR, pyrosequencing and next‐generation sequencing. Hence, we report the use of an alternative method, the conformation sensitive gel electrophoresis (CSGE) for the detection of CALR mutations in BCR‐ABL1‐negative MPN patients. Methods: Forty BCR‐ABL1‐negative MPN patients' DNA: 19 polycythemia vera (PV), 7 essential thrombocytosis (ET) and 14 primary myelofibrosis (PMF), were screened for CALR mutations by CSGE. PCR primers were designed to amplify sequences spanning between exons 8 and 9 to target the mutation hotspots in CALR. Amplicons displaying abnormal CSGE profiles by electrophoresis were directly sequenced, and results were analysed by BioEdit Sequence Alignment Editor v7.2.6. CSGE results were compared with AS‐PCR and confirmed by Sanger sequencing. Results: CSGE identified 4 types of mutations; 2 PMF patients with either CALR type 1 (c.1099_1150del52) or type 2 (c.1155_1156insTTGTC), 1 ET patient with nucleotide deletion (c.1121delA) and insertion (c.1190insA) and 1 PV patient with p.K368del (c.1102_1104delAAG) and insertion (c.1135insA) inframe mutations. Three patients have an altered KDEL motif at the C‐terminal of CALR protein. In comparison, AS‐PCR only able to detect two PMF patients with mutations, either type 1 and type 2. Conclusion: CSGE is inexpensive, sensitive and reliable alternative method for the detection of CALR mutations in BCR‐ABL1‐negative MPN patients. [ABSTRACT FROM AUTHOR]

Published

2021

16. The commensal consortium of the gut microbiome is associated with favorable responses to anti-programmed death protein 1 (PD-1) therapy in thoracic neoplasms.

Author

Huihui Yin, Lu Yang, Gongxin Peng, Ke Yang, Yuling Mi, Xingsheng Hu, Xuezhi Hao, Yuchen Jiao, Xiaobing Wang, and Yan Wang

Subjects

FECAL analysis, CHEST tumors, NONPARAMETRIC statistics, KRUSKAL-Wallis Test, IMMUNE checkpoint inhibitors, SEQUENCE analysis, GUT microbiome, ELECTROPHORESIS, LOG-rank test, RETROSPECTIVE studies, RNA, HEALTH outcome assessment, MANN Whitney U Test, FISHER exact test, REGRESSION analysis, AGAR, SURVIVAL analysis (Biometry), KAPLAN-Meier estimator, DESCRIPTIVE statistics, MEMBRANE proteins, POLYMERASE chain reaction, RECEIVER operating characteristic curves, DATA analysis software, IMMUNOTHERAPY, PROPORTIONAL hazards models

Abstract

Objective: Immune checkpoint inhibitors have revolutionized cancer therapy for multiple types of solid tumors, but as expected, a large percentage of patients do not show durable responses. Biomarkers that can predict clinical responses to immunotherapies at diagnosis are therefore urgently needed. Herein, we determined the associations between baseline gut commensal microbes and the clinical treatment efficiencies of patients with thoracic neoplasms during anti-programmed death protein 1 (PD-1) therapy. Methods: Forty-two patients with advanced thoracic carcinoma who received anti-PD-1 treatment were enrolled in the study. Baseline and time-serial stool samples were analyzed using 16S ribosomal RNA gene sequencing. Tumor responses, patient progression-free survival, and overall survival were used to measure clinical outcomes. Results: The diversities of the baseline gut microbiota were similar between responders (n = 23) and nonresponders (n = 19). The relative abundances of the Akkermansiaceae, Enterococcaceae, Enterobacteriaceae, Carnobacteriaceae and Clostridiales Family XI bacterial families were significantly higher in the responder group. These 5 bacterial families acted as a commensal consortium and better stratified patients according to clinical responses (P = 0.014). Patients with a higher abundance of commensal microbes had prolonged PFS (P = 0.00016). Using multivariable analysis, the abundance of the commensal consortium was identified as an independent predictor of anti-PD-1 immunotherapy in thoracic neoplasms (hazard ratio: 0.17; 95% confidence interval: 0.05-0.55; P = 0.003). Conclusions: Baseline gut microbiota may have a critical impact on anti-PD-1 treatment in thoracic neoplasms. The abundance of gut commensal microbes at diagnosis might be useful for the early prediction of anti-PD-1 immunotherapy responses. [ABSTRACT FROM AUTHOR]

Published

2021

17. Characterization and identification of Prachinburi β0‐thalassemia: A novel‐60 kb deletion in beta globin gene related to high levels of Hb F in heterozygous state.

Author

Jomoui, Wittaya and Tepakhan, Wanicha

Subjects

*THALASSEMIA diagnosis, *REVERSE transcriptase polymerase chain reaction, *HEMOGLOBINS, *DNA, *SEQUENCE analysis, *ELECTROPHORESIS, *SYMPTOMS, *GENES, *POLYMERASE chain reaction, *DNA polymerases

Abstract

The article presents Characterization and identification of Prachinburi β0 thalassemia, and the novel-60 kb deletion in beta globin gene related to high levels of Hb F in heterozygous state. Topics discussed include β-Thalassemia is one of the most common genetic disorders in tropical and subtropical countries; and this defect is represented by decreasing (β+) or absent (β0) β-globin chain production from the β-globin gene on the chromosome.

Published

2021

18. Development of the species-specific multiplex PCR and DNA sequencing methods for rapid authentication of Isatidis Folium and its adulterants.

Author

Yung-Chuan Hsieh, Ming-Sian Wu, Hui-Chun Lee, Chia-Yun Hsieh, Shih-Shan Huang, Chia-Fen Tsai, Ya-Tze Lin, Mei-Chih Lin, Su-Hsiang Tseng, and Der-Yuan Wang

Subjects

*IN vitro studies, *DNA, *SEQUENCE analysis, *MEDICINAL plants, *HERBAL medicine, *ELECTROPHORESIS, *GENOMICS, *QUALITY control, *GENOMES, *POLYMERASE chain reaction, *CHINESE medicine

Abstract

Isatis indigotica Fort. (family Cruciferae), is an herb widely used in traditional herbal medicine and its dried leave was named "ISATIDIS FOLIUM". Baphicacanthus cusia (Ness) Bremek. and Polygonum tinctorium Ait. are commonly misused as ISATIDIS FOLIUM in Chinese Medicine pharmacy. For the purpose of being not misused, specific primers based on the sequence difference of chloroplast trnH-psbA intergenic spacer were designed and multiplex polymerase chain reaction method (multiplex PCR) was developed. In this study, 29 original herbal materials were analyzed and our results show that DNA size after multiplex PCR was able to distinguish variations between three herbs. DNA fragments of 464, 297, 170 base pairs (bps) were represented for I. indigotica and B. cusia and P. tinctorium, respectively. In conclusion, our investigations demonstrate that molecular identification method provides more accurate results for medicinal plants detection and good quality control of ISATIDIS FOLIUM. [ABSTRACT FROM AUTHOR]

Published

2021

19. Association between SLC44A4-NOTCH4 SNPs and serum lipid levels in the Chinese Han and Maonan ethnic groups.

Author

Zheng, Peng-Fei, Yin, Rui-Xing, Guan, Yao-Zong, Wei, Bi-Liu, Liu, Chun-Xiao, and Deng, Guo-Xiong

Subjects

*AGAR, *CARRIER proteins, *CELL receptors, *CHOLESTEROL, *ELECTROPHORESIS, *ETHNIC groups, *GENETIC techniques, *HIGH density lipoproteins, *LIPIDS, *LOW density lipoproteins, *POLYMERASE chain reaction, *RACE, *SEX distribution, *TRIGLYCERIDES, *HAPLOTYPES, *SINGLE nucleotide polymorphisms, *SEQUENCE analysis

Abstract

Background: The current research was to assess the relationship of the solute carrier family 44 member 4 (SLC44A4) rs577272, notch receptor 4 (NOTCH4) rs3134931 SNPs and serum lipid levels in the Han and Maonan ethnic groups. Methods: The genetic makeup of the SLC44A4 rs577272 and NOTCH4 rs3134931 SNPs in 2467 unrelated subjects (Han, 1254; Maonan,1213) was obtained by using polymerase chain reaction and restriction fragment length polymorphism technique, combined with gel electrophoresis, and confirmed by direct sequencing. Results: The genotype frequencies of SLC44A4 rs577272 and NOTCH4 rs3134931 SNPs were different between Han and Maonan populations (P < 0.05); respectively. The SLC44A4 rs577272 SNP was associated with total cholesterol (TC) and high-density lipoprotein cholesterol (HDL-C) levels in Maonan group. The NOTCH4 rs3134931 SNP was associated with triglyceride (TG) in Han; and TG and low-density lipoprotein cholesterol (LDL-C) levels in Maonan groups (P < 0.025–0.001). Stratified analysis according to gender showed that the SLC44A4 rs577272 SNP was associated with TC and HDL-C in Han and Maonan females; TC in Maonan males, meanwhile, the NOTCH4 rs3134931 SNP was associated with TG and HDL-C in Han males; TG in Han females; TG and LDL-C in Maonan males; and TG, HDL-C and LDL-C in Maonan females. Linkage disequilibrium analysis showed that the most common haplotype was rs577272G-rs3134931A (> 50%) in both Han and Maonan groups. The haplotype of rs577272G-rs3134931A was associated with TG and HDL-C in Han; and TC, TG and HDL-C in Maonan ethnic groups. Conclusions: These results suggest that the relationship among SLC44A4 rs577272, NOTCH4 rs3134931 SNPs and serum lipid parameters may vary depending on the gender and/or ethnicity/race in some populations. Haplotypes could explain more changes in serum lipid parameters than any single SNP alone particularly for TC, TG and HDL-C. [ABSTRACT FROM AUTHOR]

Published

2020

20. Detection of Haemoglobin S using Multiplex Ligation-Dependent Probe Amplification and Flow-through Hybridization Techniques: Experience in a Tertiary Hospital.

Author

WEE S. Y., HAFIZA A., AZMA R. Z., NORUNALUWAR J., AZLIN I., MALISA M. Y., QISTINA W. N., and AINOON O.

Subjects

*CAPILLARY electrophoresis, *ELECTROPHORESIS, *HEMOGLOBINS, *HIGH performance liquid chromatography, *IMMIGRANTS, *GENETIC mutation, *POLYMERASE chain reaction, *BETA-Thalassemia, *GENE expression profiling, *DESCRIPTIVE statistics, *SEQUENCE analysis, *TERTIARY care

Abstract

Haemoglobin S (HbS, α2β26Glu→Val) is a variant haemoglobin resulted from GAG→GTG mutation on codon 6 of HBB gene. HbS haemoglobinopathy is uncommon in Malaysia and mainly seen in immigrants. However, Malaysian Indians and Malays are rarely affected. This study reviewed the laboratory findings of patients with HbS and the utilization of multiplex ligation-dependent probe amplification (MLPA) and flow-through hybridization (FTH) in the detection of HbS mutation. HbS was identified and quantified by high performance liquid chromatography (HPLC), capillary electrophoresis (CE) and cellulose acetate gel electrophoresis. Molecular analysis was performed using MLPA, FTH and Sanger Sequencing. Two Africans, three Malays and two Indian individuals aged between 2-31 years were identified from our laboratory. Five patients were homozygous HbS, one was compound heterozygous HbS/β-thalassemia and one was a carrier of HbS. The patients with homozygous HbS had their haemoglobin (Hb) ranging from 7.4-10.2 g/dL with HbS and HbF levels of 58.3-94.7% and 1.5-35.5%, respectively. The Hb of compound heterozygous HbS/β-thalassaemia patients was 5.8 g/dL and was normal in heterozygous HbS. HbS, HbF and HbA2 levels for the HbS/β-thalassaemia and the carrier were 67%, 27.2% and 4.2%, and 38.6%, 0.1% and 2.8%, respectively. Both MLPA and FTH successfully detected HbS mutation in all cases but only FTH could identify the zygosity of the HbS mutation together with underlying concomitant β-thalassaemia in a single test. [ABSTRACT FROM AUTHOR]

Published

2020

21. Construction, Cloning, and Expression of CagA Recombinant Protein of Helicobacter pylori.

Author

Moghaddam, Abbas Shapouri, Mansouri, Shamseddin, Neshani, Alireza, Firoozeh, Farzaneh, Matinpur, Azade, Khaledi, Azad, and Ghazalibina, Mehran

Subjects

*BIOLOGICAL assay, *BIOTECHNOLOGY, *ELECTROPHORESIS, *ESCHERICHIA coli, *GENES, *GENETIC techniques, *HELICOBACTER pylori, *HYDROCARBONS, *IMMUNOGENETICS, *IMMUNOGLOBULINS, *POLYMERASE chain reaction, *RECOMBINANT proteins, *MICROBIAL virulence, *WESTERN immunoblotting, *BIOINFORMATICS, *SULFUR acids, *GENE expression profiling, *SEQUENCE analysis

Abstract

Background: This study aimed to assess construction and expression of CagA recombinant protein of Helicobacter pylori (H. pylori) in Escherichia coli (E. coli) BL21. Methods: Bioinformatics was used in designing the desired gene by Gene Runner. Next, the construct was subcloned to pET21b vector and this process was confirmed by Polymerase Chain Reaction (PCR), enzyme digestion and sequencing techniques. Then, it was cloned in the Escherichia coli BL21 as an expression host. Expression of protein was verified using sodium dodecyl sulfate- polyacrylamide gel electrophoresis (SDS-PAGE) and Western blotting technique. For purification of the protein, the Ni- NTA column was used. Protein concentration was determined by the Bicinchoninic Acid Protein Assay Kit (Parstoos). Finally, Western blotting was performed using CagA antibodies and normal human serum for determining immunogenicity feature with human antiserum. Results: According to the results of the present study, CagA construct was cloned into the pET21b vector and after confirmation and cloning in host expression, recombinant protein with the size of 38 kDa was successfully expressed and purified. The recombinant CagA protein showed immunogenicity characteristics with human antiserum. Conclusion: In conclusion, only 5'-end of recombinant protein CagA with high immunogenicity effects was successfully constructed, cloned and expressed. Also, CagA recombinant protein showed good immunogenicity activity with human antiserum. [ABSTRACT FROM AUTHOR]

Published

2020

22. Annual Fluctuation in Chigger Mite Populations and Orientia Tsutsugamushi Infections in Scrub Typhus Endemic Regions of South Korea.

Author

Seong Yoon Kim, Byoungchul Gill, Bong Gu Song, Hyuk Chu, Won Il Park, Hee Il Lee, E-hyun Shin, Shin-Hyeong Cho, and Jong Yul Roh

Subjects

AGRICULTURE, ANIMAL experimentation, ANIMAL diseases, ELECTROPHORESIS, GRAM-negative bacterial diseases, MICROSCOPY, MITES, POLYMERASE chain reaction, PUBLIC health surveillance, RESEARCH funding, RODENTS, SEASONS, DESCRIPTIVE statistics, SEQUENCE analysis

Abstract

Objectives: Chigger mites are vectors for scrub typhus. This study evaluated the annual fluctuations in chigger mite populations and Orientia tsutsugamushi infections in South Korea. Methods: During 2006 and 2007, chigger mites were collected monthly from wild rodents in 4 scrub typhus endemic regions of South Korea. The chigger mites were classified based on morphological characteristics, and analyzed using nested PCR for the detection of Orientia tsutsugamushi. Results: During the surveillance period, the overall trapping rate for wild rodents was 10.8%. In total, 17,457 chigger mites (representing 5 genera and 15 species) were collected, and the average chigger index (representing the number of chigger mites per rodent), was 31.7. The monthly chigger index was consistently high (> 30) in Spring (March to April) and Autumn (October to November). The mite species included Leptotrombidium pallidum (43.5%), L. orientale (18.9%), L. scutellare (18.1%), L. palpale (10.6%), and L. zetum (3.6%). L. scutellare and L. palpale populations, were relatively higher in Autumn. Monthly O. tsutsugamushi infection rates in wild rodents (average: 4.8%) and chigger mites (average: 0.7%) peaked in Spring and Autumn. Conclusion: The findings demonstrated a bimodal pattern of the incidence of O. tsutsugamushi infections. Higher infection rates were observed in both wild rodents and chigger mites, in Spring and Autumn. However, this did not reflect the unimodal incidence of scrub typhus in Autumn. Further studies are needed to identify factors, such as human behavior and harvesting in Autumn that may explain this discordance. [ABSTRACT FROM AUTHOR]

Published

2019

23. Association of DRD2 , 5-HTTLPR, and 5-HTTVNTR Gene Polymorphisms With Posttraumatic Stress Disorder in Tibetan Adolescents: A Case–Control Study.

Author

Xiao, Yingqi, Liu, Donglin, Liu, Kun, Wu, Chenxi, Zhang, Huaguo, Niu, Ying, and Jiang, Xiaolian

Subjects

*NATURAL disasters & psychology, *AGAR, *ALLELES, *CELL receptors, *CHI-squared test, *STATISTICAL correlation, *DOPAMINE antagonists, *ELECTROPHORESIS, *GENETIC polymorphisms, *POLYMERASE chain reaction, *POST-traumatic stress disorder, *QUESTIONNAIRES, *STATISTICAL hypothesis testing, *GENETIC markers, *LOGISTIC regression analysis, *CASE-control method, *DATA analysis software, *SEQUENCE analysis, *MEMBRANE transport proteins, *MANN Whitney U Test, *GENOTYPES, *ADOLESCENCE

Abstract

Background: Earthquake exposure is a source of stress, yet only a minority of survivors experience clinically meaningful disturbance in psychological function. Genetic epidemiological research has found that posttraumatic stress disorder (PTSD) symptoms are associated with genetic factors. Further research to reveal which genetic loci relate to the development of PTSD is warranted. Method: We investigated the relationships between PTSD and the dopamine D2 receptor (DRD2) gene Taq I polymorphism and the serotonin transporter gene (SCL6A4) polymorphisms 5-hydroxytryptamine transporter gene-linked polymorphic region (5-HTTLPR) and 5-HTTVNTR in 565 adolescent earthquake survivors. PTSD-positive adolescents were identified using the PTSD Checklist–Civilian Version and the Structured Clinical Interview for the Diagnostic and Statistical Manual of Mental Disorders 4. Genotypes were analyzed using the polymerase chain reaction—restriction fragment length polymorphism analysis. The Pearson χ2 test was used to investigate the differences in genotype and allele frequencies between case and control groups. Binary logistic regression analysis was performed to identify possible influencing factors for PTSD. Results: The DRD2 Taq I and 5-HTTVNTR polymorphisms had statistically significant effects on PTSD, while 5- HTTLPR did not. Specifically, the DRD2 Taq I A1 allele was highly positively correlated with PTSD, whereas the 10 allele of 5-HTTVNTR was negatively correlated. Conclusions: These data suggest that the DRD2 Taq I and 5-HTTVNTR genotypes moderate sensitivity to stress and the expression of emotional disturbance involving PTSD symptoms. These findings have important implications for PTSD etiology as well as for both primary prevention and treatment strategies. [ABSTRACT FROM AUTHOR]

Published

2019

24. The phenotypic and molecular diversity of hemoglobinopathies in India: A review of 15 years at a referral center.

Author

Nadkarni, Anita H., Gorakshakar, Ajit C., Sawant, Pratibha M., Italia, Khushnooma Y., Upadhye, Dipti S., Gorivale, Manju S., Mehta, Pallavi R., Hariharan, Priya, Ghosh, Kanjaksha, and Colah, Roshan B.

Subjects

*HEMOGLOBINOPATHY genetics, *CHROMOSOME abnormalities, *DNA, *ELECTROPHORESIS, *GENETIC polymorphisms, *HEMOGLOBINS, *HEMOGLOBINOPATHY, *HIGH performance liquid chromatography, *MOLECULAR biology, *GENETIC mutation, *NUCLEIC acid hybridization, *POLYMERASE chain reaction, *PRENATAL diagnosis, *PHENOTYPES, *ALPHA-Thalassemia, *BETA-Thalassemia, *SEQUENCE analysis, *TERTIARY care, *GENOTYPES, HEMOGLOBINOPATHY diagnosis

Abstract

Introduction: The hemoglobinopathies pose a significant health burden in India. Apart from the β thalassemias and sickle cell disorders, α thalassemias and structural hemoglobin variants are also common. Here we have reviewed the phenotypic and molecular diversity of hemoglobinopathies encountered at a referral center in western India over a period of 15 years. Materials and Methods: Screening for hemoglobinopathies was done using HPLC and cellulose acetate electrophoresis. Molecular characterization was done using Covalent Reverse Dot Blot Hybridization (CRDB), Amplification Refractory Mutation System (ARMS), GAP PCR and direct DNA sequencing. Results: The study includes 31 075 individuals who were referred for diagnosis of hemoglobinopathies and prenatal diagnosis. Of these 14 423 individuals showed various hemoglobin abnormalities. Beta genotyping in 5615 individuals showed the presence of 49 β thalassemia mutations. 143 β thalassemia heterozygotes had normal or borderline HbA2 levels. We identified three δ gene mutations (HbA2 Pellendri, HbA2 St.George, HbA2 Saurashtra) in β thalassemia heterozygotes leading to normal HbA2 levels. The commonest defects among the raised Hb F determinants were Gγ(Αγδβ)0 Indian inversion and the HPFH‐3 Indian deletion. A total of 312 individuals showed the presence of α thalassemia, of which 12.0% had a single α gene deletion (−α/αα). HbH disease was identified in 29 cases with 10 different genotypes. Alpha globin gene triplication was seen in 2.1% of β thalassemia heterozygotes with a thalassemia intermedia phenotype. Seven unusual α chain variants and eight uncommon β chain variants were identified. Conclusion: The repertoire of molecular defects seen in the different globin genes will be valuable for management and control of these disorders both in India as well as in other countries where there is a huge influx of migrant populations from India. [ABSTRACT FROM AUTHOR]

Published

2019

25. Clinical Significance of BRAF and ZEB2 Expressions in Healthy Adjacent Tissue of Bladder Cancer.

Author

Hosseini, Shima, Saidijam, Massoud, Eslami, Hamid, Soltanian, Ali Reza, Mousavi-Bahar, Seyed Habibollah, and Mahdavinezhad, Ali

Subjects

*CANCER relapse, *TISSUE physiology, *DNA analysis, *RNA analysis, *SERINE metabolism, *AGAR, *BIOMARKERS, *STATISTICAL correlation, *ELECTROPHORESIS, *GENE expression, *MOLECULAR biology, *ONCOGENES, *POLYMERASE chain reaction, *TRANSFERASES, *BENIGN prostatic hyperplasia, *DNA-binding proteins, *DATA analysis software, *THREONINE, *SEQUENCE analysis, *TUMOR risk factors, *CANCER risk factors, BLADDER tumors

Abstract

Background: Numerous molecular changes are involved in the development and progression of bladder cancer. Regular follow-up of patients is crucial due to the high recurrence rate of bladder cancer. The aim of this study is to determine the role of B-Raf proto-oncogene, serine/threonine kinase and ZEB2 expressions in onset and progression of bladder cancer. We have also investigated their relationships to pathological characteristics. Methods: We conducted this case-control study on bladder cancer and its healthy adjacent tissue, and normal bladder tissue from patients with benign prostatic hyperplasia. After extraction of total RNA and cDNA synthesis, quantitative expression analysis was performed in duplicate using real-time PCR. Changes in the gene expression were calculated according to the 2(-ΔΔCt) equation. The products were confirmed by 1% agarose gel electrophoresis and sequenced by Bioneer Company. Data was analyzed using the SPSS software (version 16). Results: There was significantly greater B-Raf proto-oncogene, serine/threonine kinase expression in 82% of bladder tumor samples compared to the adjacent tissues. In 91.1% of tumor samples, the gene expression was also significantly higher than healthy bladder tissues from patients with benign prostatic hyperplasia. We observed overexpression of B-Raf proto-oncogene, serine/threonine kinase in 61.7% of the healthy margin tissue samples compared to healthy bladder tissues of patients with benign prostatic hyperplasia (P<0.001). Expression of ZEB2 in 52.9% of the bladder tumor samples was significantly higher than healthy peripheral tissues. This increase was observed in 94.1% of tumor samples compared to healthy bladder tissues of patients with benign prostatic hyperplasia (P<0.001). Pearson correlation coefficient showed a positive relationship between B-Raf proto-oncogene, serine/threonine kinase and ZEB2 in cancerous samples (r = 0.75) and healthy margin tissue samples (r = 0.49). Conclusion: During the carcinogenesis process, molecular changes are seen in healthy margin tissue. These molecular changes may be the reason for the high recurrence rate of bladder cancer. B-Raf proto-oncogene, serine/threonine kinase can potentially be a target cancer therapy in antisense technologies. [ABSTRACT FROM AUTHOR]

Published

2019

26. TGFβ3, MSX1, and MMP3 as Candidates for NSCL±P in an Indian Population.

Author

Kumari, Priyanka, Raman, Rajiva, and Singh, Subodh Kumar

Subjects

CLEFT palate, CLEFT lip, BIOLOGICAL assay, BLOOD collection, ELECTROPHORESIS, GENES, GENETIC polymorphisms, GENETIC mutation, POLYMERASE chain reaction, PROMOTERS (Genetics), STATISTICS, TRANSCRIPTION factors, TRANSFORMING growth factors-beta, VOLUNTEERS, DATA analysis, CASE-control method, HAPLOTYPES, DESCRIPTIVE statistics, MATRIX metalloproteinases, SEQUENCE analysis, GENETICS

Abstract

Objective: To evaluate the association of transforming growth factor β3 (TGFβ3), muscle segment homeobox 1 (MSX1), Metalloproteinases 3 (MMP3), and MMP9 genes as candidates for nonsyndromic cleft lip and/or palate in an Indian population. Design: Case-control association study, mutational screening, and functional evaluation of obtained mutations. Setting: Mutational screening of the developmental genes, TGFβ3 and MSX1, along with functional evaluation and association of promoter region SNPs--one each in MMP3 and MMP9. Patients, Participants: Two hundred forty five NSCL±P cases from G. S. Memorial Plastic Surgery Hospital and Trauma Center, Varanasi and 201 healthy controls without a family history of congenital malformations from nearby schools, primary health centers, and the university hospital. Main Outcome Measure(s): Sequencing, SSCP, and PCR-RFLP were used for candidate gene screening. MatInspector and electrophoretic mobility shift assay (EMSA) were used to check the differential transcription factor binding of the variants at promoter region. Luciferase assay was used to test the transcriptional potential of the variant, and evaluation of the alternative splice site was carried out using exon-trapping experiment. Results: Metalloproteinases3 -1171 5A/6A was associated with NSCL±P, whereas MMP9 -1562 C/T did not show association. A rare variant in the promoter region of TGFβ3 (rs117462711) creates a differential binding site, confirmed by EMSA. Luciferase assay showed 3.7-fold increased expression level in mutant construct. A synonymous change in MSX1 (rs34165410) showed association with NSCL±P, which may create an alternative splice site or lead to low codon usage. Exon-trapping experiment failed to confirm alternative splicing, indicating low codon usage frequency of the mutant affecting the gene function. Conclusions: TGFβ3, MSX1, and MMP3 are candidates for NSCL±P. [ABSTRACT FROM AUTHOR]

Published

2019

27. Differential Gene Expression by RNA-Seq Analysis of the Primo Vessel in the Rabbit Lymph.

Author

Shin, Jun-Young, Choi, Sang-Heon, Choi, Da-Woon, An, Ye-Jin, Seo, Jae-Hyuk, Choi, Jong-Gu, Rho, Min-Suk, and Lee, Sang-Suk

Subjects

ANIMAL experimentation, BLOOD vessels, DNA, DYES & dyeing, ELECTROPHORESIS, GENE expression, LYMPH nodes, MONOCLONAL antibodies, HEALTH outcome assessment, POLYMERASE chain reaction, RABBITS, RESEARCH funding, RNA, VENA cava inferior, CONTROL groups, SEQUENCE analysis

Abstract

Abstract For the connectome of primo vascular system, some long-type primo vessels dyed with Alcian blue injected into inguinal nodes, abdominal node, and axially nodes were visualized, which passed over around the vena cava of the rabbit. The Alcian blue dye revealed primo vessels and colored blue in the rabbit lymph vessels. The length of long-type primo vessels was 18 cm on average, of which diameters were about 20–30 μm, and the lymph vessels had diameters of 100–150 μm. Three different tissues of pure primo vessel, mixed primo + lymph vessel, and only lymph vessel were made to undergo RNA-Seq analysis by next-generation sequencing. We also analyzed differentially expressed genes (DEGs) from the RNA-Seq data, in which 30 genes of the primo vessels, primo + lymph vessels, and lymph vessels were selected for primo marker candidates. From the plot of DEG analysis, 10 genes had remarkably different expression pattern on the Group 1 (primo vessel) vs Group 3 (lymph vessel). With Fragments Per Kilobase of exon per Million the cutoff p-value for each gene was < 0.05. Fragments Per Kilobase of exon per Million of the 10 genes such as IGHM, HLA-DRA, HIST1H41, LPL, CD36, SRGN, DGAT2, SNCG, CD48, and GPD1 for primo vessels compared with those of lymph vessels increased twice or thrice. These results suggest that the selected genes could be used for the specific marker to construct primo connectome of circuit system in the rabbit. [ABSTRACT FROM AUTHOR]

Published

2019

28. VIM/IMP carbapenemase-producing Enterobacteriaceae in Poland: epidemic Enterobacter hormaechei and Klebsiella oxytoca lineages.

Author

Izdebski, R, Baraniak, A, Żabicka, D, Sękowska, A, Gospodarek-Komkowska, E, Hryniewicz, W, Gniadkowski, M, Zabicka, D, and Sekowska, A

Subjects

*ENTEROBACTERIACEAE diseases, *CARBAPENEMASE, *EPIDEMIOLOGY, *ENTEROBACTER, *KLEBSIELLA oxytoca, *PLASMIDS, *DIAGNOSIS, *ANTIBIOTICS, *BACTERIAL proteins, *BACTERIOPHAGE typing, *COMPARATIVE studies, *DNA, *DRUG resistance in microorganisms, *ENTEROBACTERIACEAE, *EPIDEMICS, *GENES, *HYDROLASES, *KLEBSIELLA, *RESEARCH methodology, *MEDICAL cooperation, *MICROBIAL sensitivity tests, *RESEARCH, *EVALUATION research, *CARBAPENEMS, *SEQUENCE analysis, *PHARMACODYNAMICS

Abstract

Objectives: To analyse VIM/IMP-type MBL-producing Enterobacteriaceae isolates identified in Poland during 2006-12.Methods: Isolates were typed by PFGE, followed by MLST. blaVIM/IMP genes were amplified and sequenced within class 1 integrons. Their plasmidic versus chromosomal location was assessed by nuclease S1 and I-CeuI plus hybridization experiments. Plasmids were characterized by transfer assays and PCR-based replicon typing.Results: One hundred and nineteen VIM/IMP-positive Enterobacteriaceae cases were reported in Poland from the first case in 2006 until 2012. The patients were in 54 hospitals and were infected or colonized by 121 organisms, including Enterobacter cloacae complex (n = 64), Klebsiella oxytoca (n = 23), Serratia marcescens (n = 20) and Klebsiella pneumoniae (n = 11). The isolates represented numerous pulsotypes and mainly original STs, and carried eight integrons with blaVIM-1-like genes (blaVIM-1/-4/-28/-37/-40; n = 101), three with blaVIM-2 variants (blaVIM-2/-20; n = 17) and one with blaIMP-19 (n = 3). Six integrons were new, and five and two formed prevalent families of In238-like (n = 96) and In1008-like (n = 16) elements, respectively. In238 (aacA4-blaVIM-4rpt) and In1008 (blaVIM-2-aacA4) had been originally observed in Polish Pseudomonas aeruginosa, suggestive of their transfer to enterobacteria, followed by spread and diversification. Four organisms have disseminated inter-regionally, i.e. Enterobacter hormaechei ST90 with plasmidic In238/In238a integrons (n = 36), K. oxytoca ST145 with a chromosomal In237-like element (n = 18) and two subclones of E. hormaechei ST89 with In1008- or In238-type variants (n = 8 and n = 7, respectively).Conclusions: The epidemiology of VIM/IMP-producing Enterobacteriaceae in Poland has revealed a remarkable number of specific or novel characteristics of the organisms, with some possible links to other mid-southern European countries. [ABSTRACT FROM AUTHOR]

Published

2018

29. A Novel Multiplex PCR-RFLP Method for Simultaneous Genotyping of CYP3A4*4 A>G, CYP3A4*18B G>A and CYP3A4*22 C>T.

Author

ABUBAKAR, Murtala Bello, Huay Lin TAN, and Siew Hua GAN

Subjects

*DNA analysis, *ALLELES, *BREAST tumors, *CANCER patients, *COMPUTER software, *DATABASES, *ELECTROPHORESIS, *GENETIC polymorphisms, *MEDICAL protocols, *POLYMERASE chain reaction, *TEMPERATURE, *POSTMENOPAUSE, *SEQUENCE analysis, *GENOTYPES, *CYTOCHROME P-450

Abstract

Background: Cytochrome P450 3A enzymes exhibit a variety of physiological roles and have been reported to be the most predominant enzymes involved in drugs metabolism. Single nucleotide polymorphisms (SNPs) in the genes that code for these enzymes may result in functional changes that affect enzyme activity. CYP3A4 is an important enzyme in the metabolism of many important drugs used in the treatment of breast cancer. Methods: A total of 94 post-menopausal breast cancer patients were recruited for the study and their DNA was isolated for polymerase chain reaction (PCR). The primers were designed using Primer3 software with primer specificities checked via the Basic Local Alignment Tool (BLAST) database. The primer specificity, functionality and annealing temperature were first investigated using uniplex PCR protocols, followed by a single multiplex polymerase chain reaction-restriction fragment length polymorphism (PCR-RFLP) method. The digested amplification fragments were analysed by gel electrophoresis and subsequently validated by sequencing. Results: A multiplex PCR-RFLP method was successfully developed for simultaneous detection of CYP3A4*4, CYP3A4*18B and CYP3A4*22 in a population of post-menopausal breast cancer patients. Conclusion: The technique is simple, cost-effective, time-saving and can be routinely applied in the identification of SNPs and determination of allelic and genotypic frequencies of CYP3A4*4, CYP3A4*18B and CYP3A4*22. [ABSTRACT FROM AUTHOR]

Published

2018

30. Molecular characterization of predominant Streptococcus pneumoniae serotypes causing invasive infections in Canada: the SAVE study, 2011-15.

Author

Golden, Alyssa R., Adam, Heather J., Karlowsky, James A., Baxter, Melanie, Nichol, Kimberly A., Martin, Irene, Demczuk, Walter, Van Caeseele, Paul, Gubbay, Jonathan B., Lefebvre, Brigitte, Levett, Paul N., Zahariadis, George, Haldane, David, Gad, Rita, German, Gregory, Gilmour, Matthew W., Mulvey, Michael R., Hoban, Daryl J., Zhanel, George G., and Canadian Antimicrobial Resistance Alliance (CARA)

Subjects

*STREPTOCOCCUS pneumoniae, *SEROTYPES, *ANTI-infective agents, *MICROBIAL sensitivity tests, *POLYMERASE chain reaction, *ANTIBIOTICS, *BACTERIOPHAGE typing, *COMPARATIVE studies, *DRUG resistance in microorganisms, *RESEARCH methodology, *MEDICAL cooperation, *RESEARCH, *STREPTOCOCCAL diseases, *STREPTOCOCCUS, *EVALUATION research, *SEROTYPING, *SEQUENCE analysis, *PHARMACODYNAMICS

Abstract

Objectives: This study characterized the 11 most predominant serotypes of invasive Streptococcus pneumoniae infections collected by the annual SAVE study in Canada, between 2011 and 2015.Methods: A subset of the 11 most predominant serotypes (7F, 19A, 22F, 3, 12F, 11A, 9N, 8, 33F, 15A and 6C) collected by the SAVE study was analysed using PFGE and MLST, as well as PCR to identify pilus-encoding genes. WGS analyses were performed on a subset of the above isolates plus a random selection of background strains.Results: Of the predominant serotypes analysed, 7F, 33F and 19A were obtained more commonly from children <6 years of age, whereas 15A, 6C, 22F and 11A were more common in adults >65 years of age. Pneumococcal pilus PI-1 was identified in antimicrobial-susceptible serotype 15A (61/212) and <10% of 6C isolates (16/188). PI-2 was found in serotype 7F (683/701) and two-thirds of 11A isolates (162/241). Only serotype 19A-ST320 possessed both pili. Molecular and phylogenetic analyses identified serotypes 19A, 15A, 6C, 9N and 33F as highly diverse, whereas 7F, 22F and 11A demonstrated clonality. Antimicrobial resistance determinants were common within diverse serotypes, and usually similar within a clonal complex.Conclusions: Despite successful use of conjugate vaccines, S. pneumoniae remains a highly diverse organism in Canada. Several predominant serotypes, both antimicrobial susceptible and MDR, have demonstrated rapid clonal expansion or an increase in diversity. As S. pneumoniae continues to evolve in Canada, WGS will be a necessary component in the ongoing surveillance of antimicrobial-resistant and expanding clones. [ABSTRACT FROM AUTHOR]

Published

2018

31. Molecular epidemiology of NDM-1- and OXA-48-producing Klebsiella pneumoniae in an Iranian hospital: clonal dissemination of ST11 and ST893.

Author

Solgi, Hamid, Badmasti, Farzad, Giske, Christian G, Aghamohammad, Shadi, and Shahcheraghi, Fereshteh

Subjects

*MOLECULAR epidemiology, *KLEBSIELLA pneumoniae, *DRUG resistance, *MEDICAL care, *PLASMIDS, *CARBAPENEMASE, *THERAPEUTICS

Abstract

Objectives: Despite the fact that the blaOXA-48 and blaNDM-1 genes have successfully disseminated among Klebsiella pneumoniae isolates worldwide, outbreaks remain unidentified in Iran. Here we examined the molecular epidemiology of 96 carbapenem-resistant K. pneumoniae recovered from an Iranian hospital.Methods: A total of 96 non-replicate carbapenem-resistant K. pneumoniae were recovered from clinical specimens in a university hospital. Detection of ESBLs and carbapenemases produced by studied strains was performed using PCR and DNA sequencing. The bacterial isolates were assigned to clonal lineages by PFGE and MLST. In addition, plasmids were analysed by PCR-based replicon typing and conjugation assays.Results: All isolates harboured blaOXA-48 and blaNDM-1 genes together or alone. Almost all strains also carried ESBL genes. Eighty-seven isolates of K. pneumoniae were categorized into seven pulsotypes. The predominant strain clusters/pulsotypes associated with the outbreak corresponded to ST11 (48/96) and ST893 (31/96). Plasmids carrying blaOXA-48 and blaNDM-1 were successfully transferred to Escherichia coli K12 as the recipient strain. blaOXA-48 was located on IncL/M plasmids of ∼39 kb, while blaNDM-1 was carried by either an IncFII plasmid of ∼50 kb or an untypeable plasmid of ∼4 or 10 kb.Conclusions: We describe two separate outbreaks of blaOXA-48- and blaNDM-1-carrying K. pneumoniae strains associated with dissemination of the ST11 and ST893 clones, with the ICU acting as the epicentre. The spread of plasmids carrying carbapenemase genes resulting in fulminant antimicrobial resistance is a severe concern. [ABSTRACT FROM AUTHOR]

Published

2018

32. Capillary electrophoresis fragment analysis and clone sequencing in detection of dynamic mutations of spinocerebellar ataxia.

Author

CHEN Yuan-yuan, HAO Ying, ZHANG Jin, ZHANG Xin, XIE Kun-ming, DING Ming, and GU Wei-hong

Subjects

SPINOCEREBELLAR ataxia, CAPILLARY electrophoresis, GENETIC mutation, NUCLEOTIDES, POLYMERASE chain reaction, PURINES, RESEARCH evaluation, STATISTICAL reliability, SEQUENCE analysis, GENETICS

Abstract

Objective To estimate the accuracy and stability of capillary electrophoresis fragment analysis and clone sequencing in detecting dynamic mutations of spinocerebellar ataxia (SCA). Methods Capillary electrophoresis fragment analysis and clone sequencing were used in detecting trinucleotide repeated sequence of 14 SCA patients (3 cases of SCA2, 2 cases of SCA7, 7 cases of SCA8 and 2 cases of SCA17). Results Capillary electrophoresis fragment analysis of 3 SCA2 cases showed the expanded cytosine-adenine-guanine (CAG) repeats were 31, 30 and 32, and the copy numbers of 3 clone sequencing for 3 colonies in each case were 37/40/40, 37/38/39 and 38/39/40 respectively. Capillary electrophoresis fragment analysis of 2 SCA7 cases showed the expanded CAG repeats were 57 and 34, and the copy numbers of repeats were 69, 74, 75 in 3 colonies of one case, and was 45 in the other case. For the 7 SCA8 cases with the expanded cytosine-thymine-adenine (CTA)/cytosine-thymine-guanine (CTG) repeats of 99, 111, 104, 92, 89, 104 and 75, the results of clone sequencing were 97, 116, 104, 90, 90, 102 and 76 respectively. For 2 SCA17 cases with the short/expanded CAG repeats of 37/50 and 36/45, the results of clone sequencing were 51/50/52 and 45/44 for 3 and 2 colonies. Conclusions Although the higher mobility of polymerase chain reaction (PCR) products containing dynamic mutation in the capillary electrophoresis fragment analysis might cause the deviation for analysis of copy numbers, the deviation was predictable and the results were repeatable. The clone sequencing results showed obvious instability, especially for SCA2 and SCA7 genes, which might owing to their simple CAG repeats. Consequently, clone sequencing is not suited for detection of dynamic mutation, not to mention the quantitative criteria of dynamic mutation sequencing. [ABSTRACT FROM AUTHOR]

Published

2018

33. Nine Novel PAX9 Mutations and a Distinct Tooth Agenesis Genotype-Phenotype.

Author

Wong, S.-W., Han, D., Zhang, H., Liu, Y., Zhang, X., Miao, M. Z., Wang, Y., Zhao, N., Zeng, L., Bai, B., Wang, Y.-X., Liu, H., Frazier-Bowers, S. A., and Feng, H.

Subjects

HYPODONTIA, CRANIOFACIAL abnormalities, GENETIC mutation, PHENOTYPES, GENETICS of oral diseases, DISEASE risk factors, ELECTROPHORESIS, FLUORESCENT antibody technique, GENEALOGY, GENETIC techniques, POLYMERASE chain reaction, PROTEINS, RESEARCH funding, TASTE disorders, SEQUENCE analysis

Abstract

Tooth agenesis is one of the most common developmental anomalies affecting function and esthetics. The paired-domain transcription factor, Pax9, is critical for patterning and morphogenesis of tooth and taste buds. Mutations of PAX9 have been identified in patients with tooth agenesis. Despite significant progress in the genetics of tooth agenesis, many gaps in knowledge exist in refining the genotype-phenotype correlation between PAX9 and tooth agenesis. In the present study, we complete genetic and phenotypic characterization of multiplex Chinese families with nonsyndromic (NS) tooth agenesis. Direct sequencing of polymerase chain reaction products revealed 9 novel (c.140G>C, c.167T>A, c.332G>C, c.194C>A, c.271A>T, c.146delC, c.185_189dup, c.256_262dup, and c.592delG) and 2 known heterozygous mutations in the PAX9 gene among 120 probands. Subsequently, pedigrees were extended, and we confirmed that the mutations co-segregated with the tooth agenesis phenotype (with exception of families in which DNA analysis was not available). In 1 family ( n = 6), 2 individuals harbored both the PAX9 c.592delG mutation and a heterozygous missense mutation (c.739C>T) in the MSX1 gene. Clinical characterization of families segregating a PAX9 mutation reveal that all affected individuals were missing the mandibular second molar and their maxillary central incisors are most susceptible to microdontia. A significant reduction of bitter taste perception was documented in individuals harboring PAX9 mutations ( n = 3). Functional studies revealed that PAX9 haploinsufficiency or a loss of function of the PAX9 protein underlies tooth agenesis. [ABSTRACT FROM AUTHOR]

Published

2018

34. بررسی میزان بیان miRNA جهت تشخیص زودهنگام سرطان با استفاده از دروازه هاي منطقی DNA

Author

یحیی, طاهره, کاریزي, شهره زارع, and جهانیان, علی

Subjects

*BIOMARKERS, *COMPUTER-aided design, *DNA, *ELECTROPHORESIS, *LABORATORIES, *POLYMERASE chain reaction, *TUMORS, *GENE expression profiling, *FLUORESCENT dyes, *SEQUENCE analysis, *EARLY detection of cancer

Abstract

Background: DNA-based computing is an emerging research aspect that enables the in-vivo computation and decision making with significant correctness. Recent papers show that the expression level of miRNAs are related to the progress status of some diseases such as cancers and DNA computing is introduced as a low cost and concise technique for detection of these biomarkers. In this paper, DNAbased logic gates are implemented in the laboratory to detect the level of miR-21 as the biomarker of cancer. Materials and Methods: At the first, required strands for designing DNA gates are synthesized. Then, double stranded gate is generated in laboratory using a temperature gradient that followed by electrophoresis process. This double strand is the computation engine for detecting the miR-21 biomarker. miR-21 is as input in designed gate. At the end, the expression level of miR-21 is identified by measuring the generated fluorescent. Results: at the first stage, the proposed DNA-based logic gate is evaluated by using the synthesized input strands and then it is experimented on a tumor tissue. Experimental results on synthesized strands show that its detection quality/correctness is 2.5x better than conventional methods. Conclusion: Experimental results on the tumor tissues are successful and are matched with those are extracted from real time PCR results. Also, the results show that this method is significantly more suitable than real time PCR in view of time and cost. [ABSTRACT FROM AUTHOR]

Published

2017

35. Is detection of intraperitoneal exfoliated tumor cells after surgical resection of rectal cancer a prognostic factor of survival?

Author

Arstad, Christian, Refinetti, Paulo, Torgunrud Kristensen, Annette, Giercksky, Karl-Erik, Ekstrøm, Per Olaf, and Kristensen, Annette Torgunrud

Subjects

DNA analysis, CELL analysis, ELECTROPHORESIS, LONGITUDINAL method, MITOCHONDRIA, GENETIC mutation, PERITONEUM, POLYMERASE chain reaction, DESCRIPTIVE statistics, RECTUM tumors, SEQUENCE analysis, PROGNOSIS, GENETICS

Abstract

Background: The prognostic significance of free cancer cells detected in peritoneal fluid at the time of rectal surgery remains unclear. A substantial number of patients will develop metastatic disease even with successful local treatment. This prospective non-randomized study investigated the prognostic value of intraperitoneal free cancer cells harvested in peritoneal lavage after surgery for rectal cancer. Mutational hotspots in mitochondrial DNA were examined as potential molecular signatures to detect circulating intraperitoneal free cancer cells when present in primary tumor and in lavage.Methods: Point mutations in mitochondrial DNA amplifications were determined in primary tumors and corresponding exfoliated intraperitoneal free cancer cells in lavage from 191 patients with locally advanced rectal cancer scheduled for radical treatment. Mitochondrial DNA target sequences were amplified by polymerase chain reaction and base substitutions were detected by denaturant, cycling temperature capillary electrophoresis. Detection of intraperitoneal free cancer cells was correlated to survival.Results: Of 191patients analyzed, 138 (72%) were identified with somatic mitochondrial point mutations in rectal cancer tumors. From this fraction, 45 patients (33%) had positive lavage fluid with corresponding somatic mtDNA point mutations in lavage representing circulating intraperitoneal free cancer cells. There was no significant survival difference between patients identified with or without somatic mitochondrial DNA point mutations in the corresponding lavage.Conclusion: Somatic mitochondrial DNA point mutations identified in primary rectal tumors enable detection of circulating intraperitoneal free cancer cells in lavage fluid. Intraperitoneal free cancer cells harvested from lavage immediately after surgery for rectal cancer does not represent an independent prognostic factor on survival. [ABSTRACT FROM AUTHOR]

Published

2017

36. Outdoor Growth Characterization of an Unknown Microalga Screened from Contaminated Chlorella Culture.

Author

Huo, Shuhao, Shang, Changhua, Wang, Zhongming, Zhou, Weizheng, Cui, Fengjie, Zhu, Feifei, Yuan, Zhenhong, and Dong, Renjie

Subjects

*DNA analysis, *LIPID analysis, *FATTY acid analysis, *AGAR, *ALGAE, *ALKALIES, *CELL physiology, *ECOLOGY, *ELECTROPHORESIS, *BIOLOGICAL evolution, *GENETICS, *NATURE, *POLLUTION, *POLYMERASE chain reaction, *POWER resources, *RESEARCH funding, *RNA, *WATER, *WEATHER, *PHENOMENOLOGICAL biology, *DESCRIPTIVE statistics, *SEQUENCE analysis

Abstract

Outdoor microalgae cultivation process is threatened by many issues, such as pest pollution and complex, changeable weather. Therefore, it is difficult to have identical growth rate for the microalgae cells and to keep their continuous growth. Outdoor cultivation requires the algae strains not only to have a strong ability to accumulate oil, but also to adapt to the complicated external environment. Using 18S rRNA technology, one wild strain Scenedesmus sp. FS was isolated and identified from the culture of Chlorella zofingiensis. Upon contamination by Scenedesmus sp., the species could quickly replace Chlorella zofingiensis G1 and occupy ecological niche in the outdoor column photobioreactors. The results indicated that Scenedesmus sp. FS showed high alkali resistance. It also showed that even under the condition of a low inoculum rate (OD680, 0.08), Scenedesmus sp. FS could still grow in the outdoor raceway pond under a high alkaline environment. Even under unoptimized conditions, the oil content of Scenedesmus sp. FS could reach more than 22% and C16–C18 content could reach up to 79.68%, showing that this species has the potential for the biodiesel production in the near future. [ABSTRACT FROM AUTHOR]

Published

2017

37. Identification of Three Novel Splicing Variants and Expression Analysis of Chicken GPR1 Gene.

Author

Zhang, Xueyou, Xiao, Qihai, Tian, Kai, Wang, Yan, Zhao, Xiaoling, Yin, Huadong, Li, Diyan, and Zhu, Qing

Subjects

*AMINO acid analysis, *DNA analysis, *RNA analysis, *ANIMAL experimentation, *CELL receptors, *ELECTROPHORESIS, *BIOLOGICAL evolution, *GENE expression, *GENETICS, *GENETIC techniques, *LIPIDS, *RESEARCH methodology, *OVARIES, *POLYMERASE chain reaction, *POULTRY, *PROBABILITY theory, *RESEARCH funding, *STATISTICS, *TISSUE culture, *DATA analysis, *DATA analysis software, *GENE expression profiling, *DESCRIPTIVE statistics, *SEQUENCE analysis, *ONE-way analysis of variance

Abstract

GPR1 is a G protein-coupled receptor that plays critical roles in eukaryotic cells: typically, response to glucose stimulation, lipid accumulation, and transmitting nutrition signals to cAMP pathway. However, the alternative splicing of the GPR1 gene and its expression pattern in chicken tissues and ovarian follicles were unknown. In our current study, we used RACE-PCR to identify three GPR1 variants, including the full-length variant (GPR1-va1) and two alternatively spliced variants (GPR1-va2, GPR1-vb). Quantitative real-time PCR examined the expression pattern of GPR1 mRNA in chicken tissues and ovarian follicles. The result reveals that the coding sequence of the three variants cDNA is 1053, 1053, and 627 bp in length, encoding 350, 350, and 208 amino acids, respectively. The three variants of GPR1 show similar tissue distributions; GPR1 expression was abundant in the abdominal fat, lung, and heart. With the follicular development, the expression of GPR1 gene gradually increased, and GPR1-va1 and GPR1-va2 spliced variants expression in F2 were significantly higher than in F5, F4, and prehierarchical follicles (P<0.05). Taken together, we found three novel variants of GPR1, and the results of GPR1 expression profiling in adipose tissues and ovarian follicles suggest that GPR1 may play a significant role in the lipid accumulation and progression of follicular development. [ABSTRACT FROM AUTHOR]

Published

2017

38. Emerging Perils of Extended Spectrum β-Lactamase Producing Enterobacteriaceae Clinical Isolates in a Teaching Hospital of Nepal.

Author

Parajuli, Narayan Prasad, Maharjan, Pooja, Joshi, Govardhan, and Khanal, Puspa Raj

Subjects

*DNA analysis, *ACADEMIC medical centers, *ANTIBIOTICS, *BACTERIAL diseases, *DRUG resistance in microorganisms, *ELECTROPHORESIS, *ENTEROBACTERIACEAE, *ESCHERICHIA coli, *GENES, *HOSPITALS, *HYDROLASES, *KLEBSIELLA, *MICROBIAL sensitivity tests, *POLYMERASE chain reaction, *URINARY organs, *PHENOTYPES, *DISEASE prevalence, *CROSS-sectional method, *DATA analysis software, *DESCRIPTIVE statistics, *SEQUENCE analysis, *GENOTYPES

Abstract

Introduction. Infections due to extended spectrum β-lactamase producing Enterobacteriaceae are on the rise. They pose serious public health problems due to their resistance to large number of antibiotics. However, little is known about the genotypes of ESBL from Nepal. Therefore, the study presents results of phenotypic and molecular characterization of ESBL producing Escherichia coli and Klebsiella spp. isolated from various clinical specimens in a tertiary care teaching hospital of Nepal. Methods. A total of 172 Enterobacteriaceae clinical isolates recovered from various clinical specimens were analyzed for their antibiotic susceptibility test. Detection of ESBLs was carried out using combination disk test and multiplex PCR for their genotypes (CTX-M, SHV, and TEM). Results. Out of 172 clinical isolates, 70 (40.6%) of them were found ESBL producers. The major source of ESBL producers was urinary tract samples and the highest ESBL production was observed in Escherichia coli (46.5%). Among ESBL genotypes, CTX-M (91.4%) was most predominant, followed by TEM (65.7%) and SHV (11.4%) in both of the isolates. Conclusions. High level of drug resistance and ESBL production was observed among the clinical isolates. There is a need for longitudinal and nationwide surveillance for drug resistance in clinical isolates and antimicrobial stewardship is necessary to guide the appropriate and judicious antibiotic use. [ABSTRACT FROM AUTHOR]

Published

2016

39. Detection of Natural Toxoplasma gondii Infection in Chicken in Thika Region of Kenya Using Nested Polymerase Chain Reaction.

Author

Mose, John Mokua, Kagira, John Maina, Karanja, Simon Muturi, Ngotho, Maina, Kamau, David Muchina, Njuguna, Adele Nyambura, and Maina, Naomi Wangari

Subjects

*DNA analysis, *AGRICULTURE, *ANIMAL diseases, *ANIMAL experimentation, *BRAIN, *CHI-squared test, *CONFIDENCE intervals, *ELECTROPHORESIS, *RESEARCH methodology, *POLYMERASE chain reaction, *POULTRY, *PROTOZOAN diseases, *RESEARCH funding, *TISSUE culture, *DISEASE prevalence, *CROSS-sectional method, *DATA analysis software, *DESCRIPTIVE statistics, *SEQUENCE analysis, *DIAGNOSIS

Abstract

The detection of Toxoplasma gondii in free-range chickens is a good indicator of possible risk to human beings. The aim of this study was to investigate the occurrence of T. gondii in free-range chicken using polymerase chain reaction (PCR). Brain samples from 105 free-range chickens from three administrative areas in Thika region, Kenya, were collected, DNA-extracted, and analyzed using PCR to detect presence of T. gondii. The overall prevalence of T. gondii in all the three areas was 79.0% (95% CI: 70.0–86.4%) and the prevalence across the three areas was not significantly different (P=0.5088; χ2=1.354). Female chickens had higher (79.4%) prevalence than males (78.6%), although the difference was not significant (P=0.922, χ2 = 0.01). However, chickens that were more than 2 years old had significantly (P=0.003; χ2 = 11.87) higher prevalence compared to younger ones. The study indicates that there was a high occurrence of T. gondii infection in free-range chickens from Thika region and that the infection rate is age dependent. Further studies should be carried out to determine the possible role of roaming chickens in the epidemiology of the disease among humans in the area. [ABSTRACT FROM AUTHOR]

Published

2016

40. Characterization of South American Snails of the Genus Biomphalaria (Basommatophora: Planorbidae) and Schistosoma mansoni (Platyhelminthes: Trematoda) in Molluscs by PCR-RFLP.

Author

Caldeira, Roberta Lima, Teodoro, Tatiana Maria, Jannotti-Passos, Liana Konovaloff, Lira-Moreira, Pollanah M., Goveia, Christiane De Oliveira, and Carvalho, Omar dos Santos

Subjects

*SCHISTOSOMIASIS diagnosis, *DNA analysis, *MOLLUSK classification, *ANIMAL experimentation, *DISSECTION, *ELECTROPHORESIS, *GENETIC polymorphisms, *MOLLUSKS, *POLYMERASE chain reaction, *RESEARCH funding, *TREMATODA, *SEQUENCE analysis

Abstract

The identification of snails of the genus Biomphalaria can be done using morphological characteristics which depends on the size of the snails and skill and knowledge of researcher. These methods sometimes are not adequate for identification of species. The PCR-RFLP, using the ITS region of the rDNA, has been used to identify Brazilian species of the genus Biomphalaria. Nevertheless, there is a lack of information about snails from other Latin American countries. In addition, some snails may be infected by Schistosoma mansoni and when submitted to PCR-RFLP they show molecular profiles different from those previously standardized for the other mollusc species. In this work the molecular profiles of 15 species and the subspecies were established by PCR-RFLP of ITS-rDNA with the enzyme DdeI. Moreover, the molecular profiles of host species, B. glabrata, B. straminea, B. tenagophila, and B. prona, infected by S. mansoni were also established. The molluscs were dissected to permit morphological identification. These results contribute to a correct identification of snails of the genus Biomphalaria and detection of these snails infected by S. mansoni. [ABSTRACT FROM AUTHOR]

Published

2016

41. Polymorphism of 41 kD Flagellin Gene and Its Human B-Cell Epitope in Borrelia burgdorferi Strains of China.

Author

Liu, Huixin, Liu, Wei, Hou, Xuexia, Zhang, Lin, Wan, Kanglin, and Hao, Qin

Subjects

*AMINO acid analysis, *LYME disease diagnosis, *ANTIGENS, *B cells, *BACTERIAL proteins, *ELECTROPHORESIS, *BIOLOGICAL evolution, *GENES, *GENETIC polymorphisms, *GENETICS, *GENETIC techniques, *GRAM-negative bacteria, *GENETIC mutation, *POLYMERASE chain reaction, *RESEARCH funding, *SERODIAGNOSIS, *DATA analysis software, *SEQUENCE analysis, *GENOTYPES

Abstract

The 41 kD flagellin of Borrelia burgdorferi (B. burgdorferi) is a major component of periplasmic flagellar filament core and a good candidate for serodiagnosis in early stage of Lyme disease. Here, we chose 89 B. burgdorferi strains in China, amplified the gene encoding the 41 kD flagellin, and compared the sequences. The results showed that genetic diversity presented in the 41 kD flagellin genes of all 89 strains among the four genotypes of B. burgdorferi, especially in the genotype of B. garinii. Some specific mutation sites for each genotype of the 41 kD flagellin genes were found, which could be used for genotyping B. burgdorferi strains in China. Human B-cell epitope analysis showed that thirteen of 15 nonsynonymous mutations occurred in the epitope region of 41 kD flagellin and thirty of 42 B-cell epitopes were altered due to all 13 nonsynonymous mutations in the epitope region, which may affect the function of the antigen. Nonsynonymous mutations and changed human B-cell epitopes exist in 41 kD flagellin of B. burgdorferi sensu lato strains; these changes should be considered in serodiagnosis of Lyme disease. [ABSTRACT FROM AUTHOR]

Published

2016

42. Microcystin Biosynthesis and mcyA Expression in Geographically Distinct Microcystis Strains under Different Nitrogen, Phosphorus, and Boron Regimes.

Author

Srivastava, Ankita, Ko, So-Ra, Ahn, Chi-Yong, Oh, Hee-Mock, Ravi, Alok Kumar, and Asthana, Ravi Kumar

Subjects

*BACTERIAL metabolism, *AGAR, *ANALYSIS of variance, *BACTERIAL physiology, *BACTERIAL toxins, *CELL division, *CELLULAR signal transduction, *ELECTROPHORESIS, *GENE expression, *MICROBIAL genetics, *MICROBIOLOGICAL techniques, *MULTIVARIATE analysis, *NITROGEN, *NUTRITIONAL requirements, *PEPTIDES, *PHOSPHORUS, *POLYMERASE chain reaction, *RESEARCH funding, *TRACE elements, *AQUATIC microbiology, *REVERSE transcriptase polymerase chain reaction, *DATA analysis software, *SEQUENCE analysis, *PHYSIOLOGY

Abstract

Roles of nutrients and other environmental variables in development of cyanobacterial bloom and its toxicity are complex and not well understood. We have monitored the photoautotrophic growth, total microcystin concentration, and microcystins synthetase gene (mcyA) expression in lab-grown strains of Microcystis NIES 843 (reference strain), KW (Wangsong Reservoir, South Korea), and Durgakund (Varanasi, India) under different nutrient regimes (nitrogen, phosphorus, and boron). Higher level of nitrogen and boron resulted in increased growth (avg. 5 and 6.5 Chl a mg/L, resp.), total microcystin concentrations (avg. 1.185 and 7.153 mg/L, resp.), and mcyA transcript but its expression was not directly correlated with total microcystin concentrations in the target strains. Interestingly, Durgakund strain had much lower microcystin content and lacked microcystin-YR variant over NIES 843 and KW. It is inferred that microcystin concentration and its variants are strain specific. We have also examined the heterotrophic bacteria associated with cyanobacterial bloom in Durgakund Pond and Wangsong Reservoir which were found to be enriched in Alpha-, Beta-, and Gammaproteobacteria and that could influence the bloom dynamics. [ABSTRACT FROM AUTHOR]

Published

2016

43. Expression of resistance gene analogs in woodland strawberry ( Fragaria vesca) during infection with Phytophthora cactorum.

Author

Chen, Xiao-Ren, Brurberg, May, Elameen, Abdelhameed, Klemsdal, Sonja, and Martinussen, Inger

Subjects

*STRAWBERRIES, *PHYTOPHTHORA cactorum, *POLYMERASE chain reaction, *ELECTROPHORESIS, *SEQUENCE analysis

Abstract

Important losses in strawberry production are often caused by the oomycete Phytophthora cactorum, the causal agent of crown rot. However, very limited studies at molecular levels exist of the mechanisms related to strawberry resistance against this pathogen. To begin to rectify this situation, a PCR-based approach (NBS profiling) was used to isolate strawberry resistance gene analogs (RGAs) with altered expression in response to P. cactorum during a time course (2, 4, 6, 24, 48, 96 and 192 h post-infection). Twenty-three distinct RGA fragments of the NB-LRR type were identified from a resistance genotype (Bukammen) of the wild species Fragaria vesca. The gene transcriptional profiles after infection showed that the response of most RGAs was quicker and stronger in the resistance genotype (Bukammen) than in the susceptible one (FDP821) during the early infection stage. The transcriptional patterns of one RGA (RGA109) were further monitored and compared during the P. cactorum infection of two pairs of resistant and susceptible genotype combinations (Bukammen/FDP821 and FDR1218/1603). The 5′ end sequence was cloned, and its putative protein was characteristic of NBS-LRR R protein. Our results yielded a first insight into the strawberry RGAs responding to P. cactorum infection at molecular level. [ABSTRACT FROM AUTHOR]

Published

2016

44. Cloning, Expression, and Characterization of a Novel Thermophilic Monofunctional Catalase from Geobacillus sp. CHB1.

Author

Jia, Xianbo, Chen, Jichen, Lin, Chenqiang, and Lin, Xinjian

Subjects

*AMINO acids, *BACILLACEAE, *BIOLOGICAL assay, *BIOTECHNOLOGY, *DYNAMICS, *ELECTROPHORESIS, *ESCHERICHIA coli, *BIOLOGICAL evolution, *FERMENTATION, *GENETICS, *GENETIC techniques, *HEAT, *HYDROGEN-ion concentration, *OXIDOREDUCTASES, *POLYMERASE chain reaction, *RECOMBINANT proteins, *RESEARCH funding, *TEMPERATURE, *DATA analysis software, *DESCRIPTIVE statistics, *SEQUENCE analysis

Abstract

Catalases are widely used in many scientific areas. A catalase gene (Kat) from Geobacillus sp. CHB1 encoding a monofunctional catalase was cloned and recombinant expressed in Escherichia coli (E. coli), which was the first time to clone and express this type of catalase of genus Geobacillus strains as far as we know. This Kat gene was 1,467 bp in length and encoded a catalase with 488 amino acid residuals, which is only 81% similar to the previously studied Bacillus sp. catalase in terms of amino acid sequence. Recombinant catalase was highly soluble in E. coli and made up 30% of the total E. coli protein. Fermentation broth of the recombinant E. coli showed a high catalase activity level up to 35,831 U/mL which was only lower than recombinant Bacillus sp. WSHDZ-01 among the reported catalase production strains. The purified recombinant catalase had a specific activity of 40,526 U/mg and Km of 51.1 mM. The optimal reaction temperature of this recombinant enzyme was 60°C to 70°C, and it exhibited high activity over a wide range of reaction temperatures, ranging from 10°C to 90°C. The enzyme retained 94.7% of its residual activity after incubation at 60°C for 1 hour. High yield and excellent thermophilic properties are valuable features for this catalase in industrial applications. [ABSTRACT FROM AUTHOR]

Published

2016

45. Expression and Purification of C-Peptide Containing Insulin Using Pichia pastoris Expression System.

Author

Baeshen, Mohammed N., Bouback, Thamer A. F., Alzubaidi, Mubarak A., Bora, Roop S., Alotaibi, Mohammed A. T., Alabbas, Omar T. O., Alshahrani, Sultan M., Aljohani, Ahmed A. M., Munshi, Rayan A. A., Al-Hejin, Ahmed, Ahmed, Mohamed M. M., Redwan, Elrashdy M., Ramadan, Hassan A. I., Saini, Kulvinder S., and Baeshen, Nabih A.

Subjects

*INSULIN therapy, *TREATMENT of diabetes, *AMINOGLYCOSIDES, *ANIMAL experimentation, *BIOTECHNOLOGY, *C-peptide, *DNA, *ELECTROPHORESIS, *ENZYME-linked immunosorbent assay, *GENETIC techniques, *TYPE 1 diabetes, *MICE, *POLYMERASE chain reaction, *PROINSULIN, *RECOMBINANT proteins, *RESEARCH funding, *WESTERN immunoblotting, *YEAST, *DESCRIPTIVE statistics, *SEQUENCE analysis, *IN vivo studies, *THERAPEUTICS

Abstract

Increase in the incidence of Insulin Dependent Diabetes Mellitus (IDDM) among people from developed and developing countries has created a large global market for insulin. Moreover, exploration of new methods for insulin delivery including oral or inhalation route which require very high doses would further increase the demand of cost-effective recombinant insulin. Various bacterial and yeast strains have been optimized to overproduce important biopharmaceuticals. One of the approaches we have taken is the production of recombinant human insulin along with C-peptide in yeast Pichia pastoris. We procured a cDNA clone of insulin from Origene Inc., USA. Insulin cDNA was PCR amplified and cloned into yeast vector pPICZ-α. Cloned insulin cDNA was confirmed by restriction analysis and DNA sequencing. pPICZ-α-insulin clone was transformed into Pichia pastoris SuperMan5 strain. Several Zeocin resistant clones were obtained and integration of insulin cDNA in Pichia genome was confirmed by PCR using insulin specific primers. Expression of insulin in Pichia clones was confirmed by ELISA, SDS-PAGE, and Western blot analysis. In vivo efficacy studies in streptozotocin induced diabetic mice confirmed the activity of recombinant insulin. In conclusion, a biologically active human proinsulin along with C-peptide was expressed at high level using Pichia pastoris expression system. [ABSTRACT FROM AUTHOR]

Published

2016

46. Microsatellite Length Scoring by Single Molecule Real Time Sequencing – Effects of Sequence Structure and PCR Regime.

Author

Liljegren, Mikkel Meyn, de Muinck, Eric Jacques, and Trosvik, Pål

Subjects

*MICROSATELLITE repeats, *SINGLE molecules, *NUCLEOTIDE sequence, *DNA replication, *ELECTROPHORESIS

Abstract

Microsatellites are DNA sequences consisting of repeated, short (1–6 bp) sequence motifs that are highly mutable by enzymatic slippage during replication. Due to their high intrinsic variability, microsatellites have important applications in population genetics, forensics, genome mapping, as well as cancer diagnostics and prognosis. The current analytical standard for microsatellites is based on length scoring by high precision electrophoresis, but due to increasing efficiency next-generation sequencing techniques may provide a viable alternative. Here, we evaluated single molecule real time (SMRT) sequencing, implemented in the PacBio series of sequencing apparatuses, as a means of microsatellite length scoring. To this end we carried out multiplexed SMRT sequencing of plasmid-carried artificial microsatellites of varying structure under different pre-sequencing PCR regimes. For each repeat structure, reads corresponding to the target length dominated. We found that pre-sequencing amplification had large effects on scoring accuracy and error distribution relative to controls, but that the effects of the number of amplification cycles were generally weak. In line with expectations enzymatic slippage decreased proportionally with microsatellite repeat unit length and increased with repetition number. Finally, we determined directional mutation trends, showing that PCR and SMRT sequencing introduced consistent but opposing error patterns in contraction and expansion of the microsatellites on the repeat motif and single nucleotide level. [ABSTRACT FROM AUTHOR]

Published

2016

47. Diagnosis of Xeroderma Pigmentosum Groups A and C by Detection of Two Prevalent Mutations in West Algerian Population: A Rapid Genotyping Tool for the Frequent XPC Mutation c.1643_1644delTG.

Author

Bensenouci, Salima, Louhibi, Lotfi, De Verneuil, Hubert, Mahmoudi, Khadidja, and Saidi-Mehtar, Nadhira

Subjects

*DNA analysis, *GENETIC mutation, *SEQUENCE analysis, *ELECTROPHORESIS, *GENOTYPES, *ALGERIANS, *DESCRIPTIVE statistics, *GENETIC techniques, *POLYMERASE chain reaction, *DATA analysis software, *XERODERMA pigmentosum

Abstract

Xeroderma pigmentosum (XP) is a rare autosomal recessive disorder. Considering that XP patients have a defect of the nucleotide excision repair (NER) pathway which enables them to repair DNA damage caused by UV light, they have an increased risk of developing skin and eyes cancers. In the present study, we investigated the involvement of the prevalent XPA and XPC genes mutations—nonsense mutation (c.682C>T, p.Arg228X) and a two-base-pair (2 bp) deletion (c.1643_1644delTG or p.Val548Ala fsX25), respectively—in 19 index cases from 19 unrelated families in the West of Algeria. For the genetic diagnosis of XPA gene, we proceeded to PCR-RFLP. For the XPC gene, we validated a routine analysis which includes a specific amplification of a short region surrounding the 2 bp deletion using a fluorescent primer and fragment sizing (GeneScan size) on a sequencing gel. Among the 19 index cases, there were 17 homozygous patients for the 2 bp deletion in the XPC gene and 2 homozygous patients carrying the nonsense XPA mutation. Finally, XPC appears to be the major disease-causing gene concerning xeroderma pigmentosum in North Africa. The use of fragment sizing is the simplest method to analyze this 2 bp deletion for the DNA samples coming from countries where the mutation c.1643_1644delTG of XPC gene is prevalent. [ABSTRACT FROM AUTHOR]

Published

2016

48. Genetic Diversity of Eight Domestic Goat Populations Raised in Turkey.

Author

Bulut, Zafer, Kurar, Ercan, Ozsensoy, Yusuf, Altunok, Vahdettin, and Nizamlioglu, Mehmet

Subjects

*CLASSIFICATION of mammals, *DNA analysis, *ALLELES, *ANIMAL experimentation, *ELECTROPHORESIS, *GENETICS, *POLYMERASE chain reaction, *PROBABILITY theory, *RESEARCH funding, *DATA analysis software, *DESCRIPTIVE statistics, *SEQUENCE analysis, *GENOTYPES

Abstract

The objective of this study was to determine the intra- and intergenetic diversities of eight different goat populations in Turkey including Hair, Angora, Kilis, Yayladag, Shami, Honamli, Saanen, and Alpine. A total of 244 DNA samples were genotyped using 11 microsatellites loci. The genetic differentiation between breeds was considerable as a result of the statistically significant (P<0.001) pairwise FST values of each pair of breeds. Exceptionally, FST values calculated for Honamli and Hair breeds were statistically nonsignificant (P>0.05). Heterozygosity values ranged between 0.62 and 0.73. According to the structure and assignment test, Angora and Yayladag goats were assigned to the breed they belong to, while other breeds were assigned to two or more different groups. Because this study for the first time presented genetic data on the Yayladag goat, results of structure analysis and assigned test suggest that further analyses are needed using additional and different molecular markers. [ABSTRACT FROM AUTHOR]

Published

2016

49. A <italic>KLF1</italic> gene mutation causes β‐thalassemia minor in a Chinese family.

Author

Huang, L.‐Y., Li, J., Zhang, Y., and Li, D.‐Z.

Subjects

*BETA-Thalassemia, *ELECTROPHORESIS, *GENEALOGY, *GENETIC techniques, *GENETIC mutation, *POLYMERASE chain reaction, *TRANSCRIPTION factors, *SEQUENCE analysis, *GENETICS

Published

2018

50. Detection and analysis of the cause of false-tetra-allelic patterns of locus D10S1435 at the sequence level

Author

Yongsong Zhou, Qiong Lan, Yuxin Guo, Bofeng Zhu, Weian Du, Yating Fang, and Tong Xie

Subjects

Electrophoresis, Genotyping Techniques, Sequence analysis, Locus (genetics), Biology, Nucleic Acid Denaturation, Polymerase Chain Reaction, 01 natural sciences, Pathology and Forensic Medicine, 03 medical and health sciences, 0302 clinical medicine, Gene Frequency, Humans, False Positive Reactions, 030216 legal & forensic medicine, Typing, Allele, Genotyping, Genetics, 010401 analytical chemistry, Nucleic acid sequence, Sequence Analysis, DNA, Amplicon, DNA Fingerprinting, 0104 chemical sciences, GC-content, Microsatellite Repeats

Abstract

A number of artifacts produced in forensic DNA typing make the interpretation more complicated and even lead to typing errors. Here, we reported the cause of false-tetra-allelic patterns of STR locus D10S1435 at the sequence level. To confirm the true genotyping, the sample with four allelic peaks was re-amplified and sequenced. The amplicon sequences of D10S1435, D20S482, D6S1017, and D10S1248 loci were analyzed by software BioXM and RNAstructure. We successfully reproduced the four-peak phenomenon by adding various concentration of magnesium chloride into the loading mixtures to simulate the suboptimal electrophoresis conditions. The false four allelic peaks may be caused by the specific nucleotide sequence of locus D10S1435 which tends to form secondary structures under the suboptimal electrophoresis conditions. The relatively high GC content and extremely uneven distribution give the amplicon a potency to resist complete denaturation at the phase of sample preparation and a tendency to form intra- and intermolecular secondary structures during post-injection.

Published

2019