Your search keyword '"Plasmid Vectors"' showing total 188 results

1. Hepatocyte Growth Factor and Betacellulin Gene Expression for Treating Diabetes: In vitro analysis.

Author

Desai, Yash, Patel, Micky, and Panakanti, Ravikiran

Subjects

*HEPATOCYTE growth factor, *GENE expression, *CELL death, *GENETIC vectors, *DIABETES, *ISLANDS of Langerhans

Abstract

Background: Diabetes mellitus is a fast spreading metabolic disease in both developed and developing countries owing to genetic predisposition, lifestyle and or environmental conditions. Recombinant insulin used for managing diabetes has been approved in 1985, but till now there has been no cure. Insulin cannot help the patients who become resistant to it. Islet transplantation has been developed in 2001 and can become a possible cure for Diabetes. Gene therapy can be beneficial in ameliorating the functionality and survival of islets post-transplantation. Plasmid vectors pcDNA3.1 BTC and pcDNA3.1 HGF can help with proliferation and protection of islet cells from apoptosis. Methods: Plasmid vectors encoding genes Betacellulin (BTC) and Hepatocyte growth factor (HGF) were constructed and the gene expression, caspase -3 and cell viability assays were done to assess the activity of these vectors. Results: pcDNA3.1 BTC and pcDNA3.1 HGF showed time dependent increase in expression of BTC and HGF following transfection in rat insulinoma (RIN-5mF) cells by forming complexes with lipofectamine-3000. There was no toxicity associated with the use of lipofectamine-3000 and the expression of BTC and HGF seemed to protect them from cytokine mediated apoptosis. Conclusion: The use of viral vectors is fraught with challenges especially with regards to their safety. Hence, we used plasmid vectors to express therapeutic genes Betacellulin and Hepatocyte growth factor and the use of these vectors on RIN-m5F cells showed that they could protect them from apoptosis mediated cell death and can enhance their function and survival. [ABSTRACT FROM AUTHOR]

Published

2022

2. Maintenance of Plasmid Expression in vivo Depends Primarily on the CpG Contents of the Vector and Transgene.

Author

Bruter, A. V., Kalashnikova, M. V., Prytyko, A. P., and Belyavsky, A. V.

Subjects

*TRANSGENE expression, *MESENCHYMAL stem cells, *LEG muscles, *ALKALINE phosphatase, *GENE therapy, *SKELETAL muscle

Abstract

Plasmid-mediated gene therapy, being a safe and relatively inexpensive therapeutic strategy, is plagued by a fast silencing of transgene expression. The silencing severely reduces the long-term efficiency of plasmid vectors. We have earlier constructed a low-CpG pMBR2 plasmid vector supporting prolonged expression of transgenes in mesenchymal stem cells in vitro. Long-term expression from the pMBR2 vector was studied for the wild-type mouse secreted alkaline phosphatase gene (mSEAPTwt) and its version devoid of CpGs (mSEAP0) after vector electroporation into mouse hindlimb muscles and hydrodynamic delivery to the liver. The mSEAP levels in the blood were measured over one year. With the pMBR2-mSEAP0 construct, the mSEAP levels in leg muscles increased more than 2.5-fold in the first two months and remained higher than the initial level until the end of the experiment. Far lower expression levels were observed with the control pCDNA3.1-mSEAP0 construct. Expression from pMBR2-mSEAPwt decreased to about 40% after 6 months and remained at similar levels thereafter. In the mouse liver, expression from pMBR2-mSEAP0 was approximately halved within the first 18 weeks and then decrease slowly to the final 17% level. Expression from pMBR2-mSEAPwt initially dropped to 18% and remained at approximately 10% thereafter. In contrast, expression from pCDNA3.1-mSEAP0 sharply dropped to 5% after 2 weeks and remained at nearly zero levels throughout the rest of the experiment. Thus, both vector and transgene should have significantly reduced CpG contents to ensure prolonged plasmid-mediated expression in the liver, while minimizing the vector CpG content is sufficient for expression in skeletal muscles. The results suggested additionally that the localization of S/MAR elements within the transcription unit, in contrast to their outside location, results in significant reduction of the level of secreted, but not cytoplasmic, proteins. [ABSTRACT FROM AUTHOR]

Published

2020

3. The functions and mechanisms of sequence differences of DGAT1 gene on milk fat synthesis between dairy cow and buffalo.

Author

Bhattarai, Dinesh, Dad, Rahim, Worku, Tesfay, Xu, Sutong, Ullah, Farman, Zhang, Min, Liang, Xianwei, Den, Tingxian, Fan, Mingxia, and Zhang, Shujun

Subjects

FAT content of milk, COWS, CHO cell, REPORTER genes, EPITHELIAL cells

Abstract

In this research communication we describe the DGAT1 sequence and promoter region in dairy cows and buffalo and compare the activities of DGAT1 between the two species in order to increase knowledge of the cause of milk fat variation. pGL-3 basic vectors were used to construct the reporter gene. Based on the predicted promoter region, 4 truncated plasmid vectors were constructed in cow-DGAT1 and 3 plasmid vectors in buffalo-DGAT1. Each reporter plasmid was transfected into the bovine mammary epithelial cell (BMEC), 293T cell, and CHO cells to analyze the activity using Dual-Luciferase Reporter Assay System. The results show that the region between −93 to −556 bp was essential for cow promoter activity while −84 to −590 bp was essential for buffalo promoter activity revealing these regions contain core promoter. The buffalo has higher promoter activity than cow yet it was not statistically significant. Comparison of candidate mutation K232A between cow and buffalo population revealed the presence of both the allelic population in dairy cows (lysine and alanine) however, only K (lysine) allelic amino acid was found in buffalo population. The absence of the alanine allelic population from buffalo explains the higher fat content of buffalo milk. [ABSTRACT FROM AUTHOR]

Published

2020

4. Analysis of Human Genome for Viral Proto - Oncogenes.

Author

FRANCIS, TWINKLE, N. P., MURALIDHARAN, and ANJALI, A. K

Subjects

*HUMAN genome, *VIRAL genomes, *CELL death, *CELL death inhibition, *ONCOGENES, *CHROMOSOME structure, *CELL division

Abstract

The human genome consists of multiple dispersed nucleotide fragments and sequences that are related to the proto-oncogene MOS and to pro retroviral sequences which are in light text position to each other. From sequencing appropriate closed fragments of human DNA in phage, studies have shown that plasmid vectors follow one of the regions, NV-1 and Cl-1. Oncogenes show an increased production of these proteins that leads to increased cell division, decreased cell differentiation and cell death inhibition which define the phenotype of cancer cells. Potential oncogenicity of a normal human genome undergoes two disputed influences: it increases due to proto-oncogene amplification and decreases due to inactivation of some of them. These genes should be active in development and that it may be positive to identify their roles by examination of embryonic tissues. Hence, this detailed study helps in the understanding of certain regulatory processes that may provide new approaches to therapeutics that have a significant impact on aberrant chromosomal structures. [ABSTRACT FROM AUTHOR]

Published

2020

5. Constructing Clinically Applicable Plasmids for Cancer Gene Therapy

Author

Kamensek, U., Tesic, N., Sersa, G., Cemazar, M., MAGJAREVIC, Ratko, Editor-in-chief, Ladyzynsk, Piotr, Series editor, Ibrahim, Fatimah, Series editor, Lacković, Igor, Series editor, Rock, Emilio Sacristan, Series editor, Jarm, Tomaz, editor, and Kramar, Peter, editor

Published

2016

6. Functional and immunological aspects of growth hormone gene transfer into muscle cells

Author

MacColl, Gavin Stuart

Subjects

572.8, Plasmid vectors, DNA, Autoimmunity

Abstract

Several practical aspects of gene transfer into muscle using plasmid vectors were studied in this thesis. First, the influence of promoter sequences on growth hormone expression by muscle cells was studied following transfection with various plasmid constructs containing a rat growth hormone complementary DNA (GH cDNA). Second, the plasmid vector which produced the highest levels of recombinant GH in vitro was delivered by intramuscular injection into GH deficient dwarf rats, and the effects were studied. Third, the immunogenicity of plasmid vectors were studied in immunologically normal Balb/C mice, and in MRL/MpJ mice which had a genetic background for a mild autoimmunity. The findings included: 1. The combination of cytomegalovirus immediate early promoter (CMV), myosin light chain enhancer and GH cDNA (pcDNA3E-GH), generated significantly more biologically active GH in differentiated C2C12 mouse myotubes than either CMV promoter, or muscle specific promoter used individually (p<0.05). 2. Intramuscular transfer of a plasmid reporter vector was more effective in 4 week old male rats, than in older animals. Subsequent injections of pcDNA3E-GH into dwarf rats did not significantly increase weight gain, or circulating insulin like growth factor 1 (IGF-1) levels. However, immunoreactive IGF-1 was detected in the colons of 4 of 5 rats compared with only 1 of the controls, suggesting that this methodology could be used to modulate local IGF-1 production in the gastrointestinal tract. 3. MRL/MpJ mice given i.m. injections of pcDNA3E at 4, 6, 8 and 10 weeks, generated significantly higher serum anti-double stranded DNA (dsDNA) immunoglobulins, than saline injected controls (p<0.05). Additionally, sera from 6 of the 7 of the plasmid injected MRL/MpJ mice contained anti-cell nuclear immunoglobulins, compared with 2 control sera. No increase in dsDNA antibodies was observed in Balb/C mice injected with pcDNA3E, or with plasmids with fewer eukaryotic sequences, suggesting that plasmid DNA injection into muscle may only alter circulating levels of anti-dsDNA antibodies in circumstances where individuals are susceptible to specific types of autoimmunity.

Published

2000

7. Investigation of sRNA-mRNA Interactions in Bacillus subtilis In Vivo.

Author

Ul Haq I, Müller P, and Brantl S

Subjects

RNA, Messenger metabolism, RNA, Bacterial metabolism, Genes, Reporter, Gene Expression Regulation, Bacterial, Bacillus subtilis genetics, Bacillus subtilis metabolism, RNA, Small Untranslated metabolism

Abstract

In this chapter, we describe in vivo methods for the analysis of interactions between an sRNA and its target mRNA in B. subtilis. All these methods have been either established or significantly improved in our group and successfully employed to characterize a number of sRNA/target mRNA systems in Bacillus subtilis. Whereas in Chap. 8, we describe a combination of in vitro methods, e.g., EMSA and RNA secondary structure probing, we focus here on the investigation of RNA-RNA interactions in vivo using compatible plasmids or chromosomal insertions and deletions, the elucidation of the mechanisms of action of regulatory sRNAs employing transcriptional and translational reporter gene fusions, as well as the determination of expression profiles, half-lives of sRNA and mRNA, and their intracellular concentrations, and, finally, the investigation of RNA chaperones that promote the sRNA/mRNA interaction. For an in-depth analysis of sRNA-mRNA interactions in B. subtilis, a combination of in vivo and in vitro methods should be applied., (© 2024. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2024

8. Apoptin Towards Safe and Efficient Anticancer Therapies

Author

Backendorf, Claude, Noteborn, Mathieu H. M., Cohen, Irun R., Series editor, Lajtha, N.S. Abel, Series editor, Lambris, John D., Series editor, Paoletti, Rodolfo, Series editor, and Grimm, Stefan, editor

Published

2014

9. Avian oncogenic herpesvirus antagonizes the cGAS-STING DNA-sensing pathway to mediate immune evasion.

Author

Li, Kai, Liu, Yongzhen, Xu, Zengkun, Zhang, Yu, Luo, Dan, Gao, Yulong, Qian, Yingjuan, Bao, Chenyi, Liu, Changjun, Zhang, Yanping, Qi, Xiaole, Cui, Hongyu, Wang, Yongqiang, Gao, Li, and Wang, Xiaomei

Subjects

*TYPE I interferons, *MAREK'S disease, *COMPUTATIONAL biology, *VIRUS diseases, *MOLECULAR biology, *T cells

Abstract

The cellular DNA sensor cGMP-AMP synthase (cGAS) detects cytosolic viral DNA via the stimulator of interferon genes (STING) to initiate innate antiviral response. Herpesviruses are known to target key immune signaling pathways to persist in an immune-competent host. Marek’s disease virus (MDV), a highly pathogenic and oncogenic herpesvirus of chickens, can antagonize host innate immune responses to achieve persistent infection. With a functional screen, we identified five MDV proteins that blocked beta interferon (IFN-β) induction downstream of the cGAS-STING pathway. Specifically, the MDV major oncoprotein Meq impeded the recruitment of TANK-binding kinase 1 and IFN regulatory factor 7 (IRF7) to the STING complex, thereby inhibiting IRF7 activation and IFN-β induction. Meq overexpression markedly reduced antiviral responses stimulated by cytosolic DNA, whereas knockdown of Meq heightened MDV-triggered induction of IFN-β and downstream antiviral genes. Moreover, Meq-deficient MDV induced more IFN-β production than wild-type MDV. Meq-deficient MDV also triggered a more robust CD8+ T cell response than wild-type MDV. As such, the Meq-deficient MDV was highly attenuated in replication and lymphoma induction compared to wild-type MDV. Taken together, these results revealed that MDV evades the cGAS-STING DNA sensing pathway, which underpins the efficient replication and oncogenesis. These findings improve our understanding of the virus-host interaction in MDV-induced lymphoma and may contribute to the development of novel vaccines against MDV infection. [ABSTRACT FROM AUTHOR]

Published

2019

10. pTcGW plasmid vectors 1.1 version: a versatile tool for Trypanosoma cruzi gene characterisation

Author

Fernanda G Kugeratski, Michel Batista, Alexandre Haruo Inoue, Bruno Dias Ramos, Marco Aurelio Krieger, and Fabricio K Marchini/

Subjects

Trypanosoma cruzi, plasmid vectors, pTcGW platform, reverse genetics, cloning, gene characterisation, Microbiology, QR1-502, Infectious and parasitic diseases, RC109-216

Abstract

The functional characterisation of thousands of Trypanosoma cruzi genes remains a challenge. Reverse genetics approaches compatible with high-throughput cloning strategies can provide the tool needed to tackle this challenge. We previously published the pTcGW platform, composed by plasmid vectors carrying different options of N-terminal fusion tags based on Gateway® technology. Here, we present an improved 1.1 version of pTcGW vectors, which is characterised by a fully flexible structure allowing an easy customisation of each element of the vectors in a single cloning step. Additionally, both N and C-terminal fusions are available with new tag options for protein complexes purification. Three of the newly created vectors were successfully used to determine the cellular localisation of four T. cruzi proteins. The 1.1 version of pTcGW platform can be used in a variety of assays, such as protein overexpression, identification of protein-protein interaction and protein localisation. This powerful and versatile tool allows adding valuable functional information to T. cruzigenes and is freely available for scientific community.

Published

2015

11. De novo biosynthesis of myricetin, kaempferol and quercetin in Streptomyces albus and Streptomyces coelicolor.

Author

Marín, Laura, Gutiérrez-del-Río, Ignacio, Entrialgo-Cadierno, Rodrigo, Villar, Claudio J., and Lombó, Felipe

Subjects

*BIOSYNTHESIS, *MYRICETIN, *QUERCETIN, *STREPTOMYCES coelicolor, *FLAVONOLS

Abstract

Flavonols are a flavonoid subfamily widely distributed in plants, including several ones of great importance in human and animal diet (apple, tomato, broccoli, onion, beans, tea). These polyphenolic nutraceuticals exert potent antimicrobial (membrane potential disruptors), antioxidant (free-radical scavengers), pharmacokinetic (CYP450 modulators), anti-inflammatory (lipoxygenase inhibitors), antiangiogenic (VEGF inhibitors) and antitumor (cyclin inhibitors) activities. Biotechnological production of these nutraceuticals, for example via heterologous biosynthesis in industrial actinomycetes, is favored since in plants these polyphenols appear as inactive glycosylated derivatives, in low concentrations or as part of complex mixtures with other polyphenolic compounds. In this work, we describe the de novo biosynthesis of three important flavonols, myricetin, kaempferol and quercetin, in the industrially relevant actinomycetes Streptomyces coelicolor and S. albus. De novo biosynthesis of kaempferol, myricetin and quercetin in actinomycetes has not been described before. [ABSTRACT FROM AUTHOR]

Published

2018

12. Metabolic engineering of <italic>Corynebacterium glutamicum</italic> for fermentative production of chemicals in biorefinery.

Author

Baritugo, Kei-Anne, Kim, Hee Taek, David, Yokimiko, Choi, Jong-il, Hong, Soon Ho, Jeong, Ki Jun, Choi, Jong Hyun, Joo, Jeong Chan, and Park, Si Jae

Subjects

*CORYNEBACTERIUM glutamicum, *FERMENTATION, *BACTERIAL metabolism, *GENETIC engineering in microbiology, *RECOMBINANT microorganisms, *SYNTHETIC biology

Abstract

Bio-based production of industrially important chemicals provides an eco-friendly alternative to current petrochemical-based processes. Because of the limited supply of fossil fuel reserves, various technologies utilizing microbial host strains for the sustainable production of platform chemicals from renewable biomass have been developed. Corynebacterium glutamicum is a non-pathogenic industrial microbial species traditionally used for l-glutamate and l-lysine production. It is a promising species for industrial production of bio-based chemicals because of its flexible metabolism that allows the utilization of a broad spectrum of carbon sources and the production of various amino acids. Classical breeding, systems, synthetic biology, and metabolic engineering approaches have been used to improve its applications, ranging from traditional amino-acid production to modern biorefinery systems for production of value-added platform chemicals. This review describes recent advances in the development of genetic engineering tools and techniques for the establishment and optimization of metabolic pathways for bio-based production of major C2-C6 platform chemicals using recombinant C. glutamicum. [ABSTRACT FROM AUTHOR]

Published

2018

13. Persistence of plasmid‐mediated expression of transgenes in human mesenchymal stem cells depends primarily on CpG levels of both vector and transgene.

Author

Bruter, Alexandra V., Kandarakov, Oleg F., and Belyavsky, Alexander V.

Abstract

Abstract: Background: Gene therapy and cell modification for clinical applications using plasmid vectors are considered to be a safe and promising strategy. One of the major problems with plasmid vector‐based constructs is a rapid decline of transgene expression in cells in vitro and in vivo. An important role of CpG motifs or bacterial vector backbone in expression silencing has been suggested. Methods: To address the effects of CpG motifs on transgene expression maintenance in stem cells in vitro, we constructed a novel pMBR2 plasmid vector containing 13 CpG motifs only. pMBR2 constructs with CpG‐free and CpG‐replete firefly luciferase inserts were introduced into cultured human adipose‐derived mesenchymal stem (MSCs) by electroporation, and luciferase expression levels were monitored for 3 weeks. Results: The pMBR2 vector with CpG‐free luciferase insert demonstrated the highest persistence of expression, whereas the wild‐type luciferase insert containing 97 CpG motifs demonstrated lower expression maintenance in the same vector. In comparison, the same inserts in the CpG‐replete pCDNA3 vector demonstrated significantly lower expression levels and only a minimal persistence of expression. β‐galactosidase and enhanced green fluorescent protein genes inserted into pMBR2 vector also demonstrated higher expression levels and better maintenance compared to the same genes in pCDNA3 vector. Conclusions: The persistence of plasmid vector expression in human MSCs is determined primarily by CpG content of both vector and transgene. The data obtained in the present study indicate that the pMBR2 vector with a minimized number of CpG motifs is appropriate for extended plasmid‐mediated expression of transgenes in MSCs and possibly other types of stem cells. [ABSTRACT FROM AUTHOR]

Published

2018

14. Molecular Basis of Stationary Phase Survival and Applications

Author

Jananee Jaishankar and Preeti Srivastava

Subjects

stationary phase promoters, stationary phase gene expression, plasmid vectors, sigma factor, stationary phase, Microbiology, QR1-502

Abstract

Stationary phase is the stage when growth ceases but cells remain metabolically active. Several physical and molecular changes take place during this stage that makes them interesting to explore. The characteristic proteins synthesized in the stationary phase are indispensable as they confer viability to the bacteria. Detailed knowledge of these proteins and the genes synthesizing them is required to understand the survival in such nutrient deprived conditions. The promoters, which drive the expression of these genes, are called stationary phase promoters. These promoters exhibit increased activity in the stationary phase and less or no activity in the exponential phase. The vectors constructed based on these promoters are ideal for large-scale protein production due to the absence of any external inducers. A number of recombinant protein production systems have been developed using these promoters. This review describes the stationary phase survival of bacteria, the promoters involved, their importance, regulation, and applications.

Published

2017

15. Molecular Basis of Stationary Phase Survival and Applications.

Author

Jaishankar, Jananee and Srivastava, Preeti

Subjects

CELL growth, GENE expression, SIGMA factor (Transcription factor)

Abstract

Stationary phase is the stage when growth ceases but cells remain metabolically active. Several physical and molecular changes take place during this stage that makes them interesting to explore. The characteristic proteins synthesized in the stationary phase are indispensable as they confer viability to the bacteria. Detailed knowledge of these proteins and the genes synthesizing them is required to understand the survival in such nutrient deprived conditions. The promoters, which drive the expression of these genes, are called stationary phase promoters. These promoters exhibit increased activity in the stationary phase and less or no activity in the exponential phase. The vectors constructed based on these promoters are ideal for large-scale protein production due to the absence of any external inducers. A number of recombinant protein production systems have been developed using these promoters. This review describes the stationary phase survival of bacteria, the promoters involved, their importance, regulation, and applications. [ABSTRACT FROM AUTHOR]

Published

2017

16. Targeted mutagenesis in a human-parasitic nematode.

Author

Gang, Spencer S., Castelletto, Michelle L., Bryant, Astra S., Yang, Emily, Mancuso, Nicholas, Lopez, Jacqueline B., Pellegrini, Matteo, and Hallem, Elissa A.

Subjects

*NEMATODE infections, *MUTAGENESIS, *CRISPRS, *CASPASES, *PHENOTYPES

Abstract

Parasitic nematodes infect over 1 billion people worldwide and cause some of the most common neglected tropical diseases. Despite their prevalence, our understanding of the biology of parasitic nematodes has been limited by the lack of tools for genetic intervention. In particular, it has not yet been possible to generate targeted gene disruptions and mutant phenotypes in any parasitic nematode. Here, we report the development of a method for introducing CRISPR-Cas9-mediated gene disruptions in the human-parasitic threadworm Strongyloides stercoralis. We disrupted the S. stercoralis twitchin gene unc-22, resulting in nematodes with severe motility defects. Ss-unc-22 mutations were resolved by homology-directed repair when a repair template was provided. Omission of a repair template resulted in deletions at the target locus. Ss-unc-22 mutations were heritable; we passed Ss-unc-22 mutants through a host and successfully recovered mutant progeny. Using a similar approach, we also disrupted the unc-22 gene of the rat-parasitic nematode Strongyloides ratti. Our results demonstrate the applicability of CRISPR-Cas9 to parasitic nematodes, and thereby enable future studies of gene function in these medically relevant but previously genetically intractable parasites. [ABSTRACT FROM AUTHOR]

Published

2017

17. Vaccines against Botulism.

Author

Sundeen, Grace and Barbieri, Joseph T.

Subjects

*BOTULISM, *SEROTYPES, *PLASMIDS, *ADENOVIRUSES, *VACCINATION, *THERAPEUTICS

Abstract

Botulinum neurotoxins (BoNT) cause the flaccid paralysis of botulism by inhibiting the release of acetylcholine from motor neurons. There are seven serotypes of BoNT (A-G), with limited therapies, and no FDA approved vaccine for botulism. An investigational formalin-inactivated penta-serotype-BoNT/A-E toxoid vaccine was used to vaccinate people who are at high risk of contracting botulism. However, this formalin-inactivated penta-serotype-BoNT/A-E toxoid vaccine was losing potency and was discontinued. This article reviews the different vaccines being developed to replace the discontinued toxoid vaccine. These vaccines include DNA-based, viral vector-based, and recombinant protein-based vaccines. DNA-based vaccines include plasmids or viral vectors containing the gene encoding one of the BoNT heavy chain receptor binding domains (HC). Viral vectors reviewed are adenovirus, influenza virus, rabies virus, Semliki Forest virus, and Venezuelan Equine Encephalitis virus. Among the potential recombinant protein vaccines reviewed are HC, light chain-heavy chain translocation domain, and chemically or genetically inactivated holotoxin. [ABSTRACT FROM AUTHOR]

Published

2017

18. Multiple UBXN family members inhibit retrovirus and lentivirus production and canonical NFκΒ signaling by stabilizing IκBα.

Author

Hu, Yani, O’Boyle, Kaitlin, Auer, Jim, Raju, Sagar, You, Fuping, Wang, Penghua, Fikrig, Erol, and Sutton, Richard E.

Subjects

*LENTIVIRUSES, *RETROVIRUS diseases, *RETROVIRUSES, *ANTIGEN receptors, *PROTEINS

Abstract

UBXN proteins likely participate in the global regulation of protein turnover, and we have shown that UBXN1 interferes with RIG-I-like receptor (RLR) signaling by interacting with MAVS and impeding its downstream effector functions. Here we demonstrate that over-expression of multiple UBXN family members decreased lentivirus and retrovirus production by several orders-of-magnitude in single cycle assays, at the level of long terminal repeat-driven transcription, and three family members, UBXN1, N9, and N11 blocked the canonical NFκB pathway by binding to Cullin1 (Cul1), inhibiting IκBα degradation. Multiple regions of UBXN1, including its UBA domain, were critical for its activity. Elimination of UBXN1 resulted in early murine embryonic lethality. shRNA-mediated knockdown of UBXN1 enhanced human immunodeficiency virus type 1 (HIV) production up to 10-fold in single cycle assays. In primary human fibroblasts, knockdown of UBXN1 caused prolonged degradation of IκBαand enhanced NFκB signaling, which was also observed after CRISPR-mediated knockout of UBXN1 in mouse embryo fibroblasts. Knockout of UBXN1 significantly up- and down-regulated hundreds of genes, notably those of several cell adhesion and immune signaling pathways. Reduction in UBXN1 gene expression in Jurkat T cells latently infected with HIV resulted in enhanced HIV gene expression, consistent with the role of UBXN1 in modulating the NFκB pathway. Based upon co-immunoprecipitation studies with host factors known to bind Cul1, models are presented as to how UBXN1 could be inhibiting Cul1 activity. The ability of UBXN1 and other family members to negatively regulate the NFκB pathway may be important for dampening the host immune response in disease processes and also re-activating quiescent HIV from latent viral reservoirs in chronically infected individuals. [ABSTRACT FROM AUTHOR]

Published

2017

19. The Impact of MicroRNA-223-3p on IL-17 Receptor D Expression in Synovial Cells.

Author

Moriya, Nozomu, Shibasaki, Seiji, Karasaki, Miki, and Iwasaki, Tsuyoshi

Subjects

*RHEUMATOID arthritis diagnosis, *AUTOIMMUNE diseases, *MICRORNA, *INTERLEUKIN-17, *GENE expression, *INFLAMMATION, *CONNECTIVE tissue cells

Abstract

Objective: Rheumatoid arthritis (RA) is an autoimmune inflammatory disease affecting joints. Elevated plasma levels of microRNA-223-3p (miR-223-3p) in patients with RA are implicated in the pathogenesis of the disease. This study aimed to analyze the functional role of miR-223-3p in the pathogenesis of RA by overexpressing miR-223-3p in synovial cell lines. Methods: Arthritis was induced in the RA model of SKG mice by injection of ß-glucan. The histopathologic features of joints were examined using hematoxylin and eosin and immunohistochemical staining. Plasma levels of miRNA were determined by panel real-time PCR analysis. Target genes of the differentially expressed miRNAs in SKG mice were analyzed using miRNA target prediction algorithms. The dual-luciferase reporter system was used to evaluate the relationship between miR-223-3p and IL-17 receptor D (IL-17RD). The activity of miR-223-3p was analyzed by transfection of plasmid vectors overexpressing miR-223-3p into IL-17RD-expressing NIH3T3 and MH7A cell lines. Il6 and Il17rd mRNA expression was analyzed by quantitative real-time PCR. IL-17RD protein expression was analyzed by western blot analysis. Results: We identified 17 upregulated miRNAs (fold change > 2.0) in plasma of SKG mice injected with ß-glucan relative to untreated SKG mice. Il17rd was identified as the candidate target gene of miR-223-3p using five miRNA target prediction algorithms. The transfection of plasmid vectors overexpressing miR-223-3p into NIH3T3 and MH7A cells resulted in the downregulation of Il17rd expression and upregulation of Il6 expression. Expression of miR-223-3p and Il6 mRNA in MH7A cells was upregulated; however, that of Il17rd mRNA was downregulated following TNF-α stimulation. IL-17RD expression in synovial tissues from SKG mice and RA patients was inversely correlated with the severity of arthritis. Conclusion: This study is the first to demonstrate that miR-223-3p downregulates IL-17RD in both mouse and human cells; miR-223-3p may contribute to the pathogenesis of RA by downregulating the expression of IL-17RD and upregulating that of IL-6 in synovial cells. [ABSTRACT FROM AUTHOR]

Published

2017

20. Karakterizacija i genetička transformacija odabranih vrsta nekonvencionalnih kvasaca iz roda Schwanniomyces

Author

Slišković, Ana and Svetec Miklenić, Marina

Subjects

genetička transformacija, nekonvencionalni kvasci, rod Schwanniomyces, plazmidi, nekonvencionalni kvasci, rod Schwanniomyces, genetička transformacija, plasmid vectors, BIOTEHNIČKE ZNANOSTI. Biotehnologija, genetic transformation, plazmidi, unconventional yeasts, genus Schwanniomyces, BIOTECHNICAL SCIENCES. Biotechnology

Abstract

Kako bi se ostvarila maksimalna efikasnost industrijskog bioprocesa, poželjno je da radni organizam bude otporan na širok raspon parametara procesnih uvjeta te da efikasno proizvodi željeni proizvod. Nekonvencionalni kvasci predstavljaju raznoliku skupinu organizama od kojih pojedine vrste prirodno posjeduju razne biotehnološki interesantne karakteristike te se sve češće koriste u proizvodnji. U skupinu nekonvencionalnih kvasaca spadaju i vrste iz roda Schwanniomyces, koje osim mogućnosti rasta na različitim izvorima ugljika pokazuju i efikasnu sekreciju proteina velike molekulske mase u podlogu. Unatoč navedenim prednostima, mnoge vrste ovog roda još uvijek nisu detaljno istražene zbog nedostatka prikladnih metoda za genetičku transformaciju i ciljane genetičke modifikacije. Stoga je cilj ovog rada bio transformirati kvasce Schwanniomyces occidentalis var. occidentalis, Schwanniomyces occidentalis var. persoonii, Schwanniomyces capriottii i Schwanniomyces vanrijiae var. yarrowii, te ispitati aktivnost ishodišta replikacije iz različitih vrsta kvasaca korištenjem plazmidnih vektora. In order to achieve the maximum efficiency of industrial bioprocesses, it is desirable for the working organism to be resistant to a wide range of process conditions and to efficiently produce the desired product. Non-conventional yeasts represent a diverse group of organisms, some species of which naturally possess various biotechnologically interesting characteristics and are increasingly used in production. The group of non-conventional yeasts also includes species from the genus Schwanniomyces, which, in addition to the ability to grow on different carbon sources, also show efficient secretion of high molecular weight proteins into the substrate. Despite the mentioned advantages, many species of this genus have not yet been investigated in detail due to the lack of suitable methods for genetic transformation and targeted genetic modification. Therefore, the aim of this work was to transform the yeast Schwanniomyces occidentalis var. occidentalis, Schwanniomyces occidentalis var. persoonii, Schwanniomyces capriottii and Schwanniomyces vanrijiae var. yarrowii, and to examine the activity of origins of replication from different yeast species using plasmid vectors.

Published

2022

21. Vectors containing streptococcal bacteriophage integrases for site-specific gene insertion

Author

McShan, W. Michael, McLaughlin, Robert E., Nordstrand, Annika, Ferretti, Joseph J., Fives-Taylor, Paula M., editor, and LeBlanc, Donald J., editor

Published

1998

22. Expression of the lncRNA Maternally Expressed Gene 3 (MEG3) Contributes to the Control of Lung Cancer Cell Proliferation by the Rb Pathway.

Author

Kruer, Traci L., Dougherty, Susan M., Reynolds, Lindsey, Long, Elizabeth, de Silva, Tanya, Lockwood, William W., and Clem, Brian F.

Subjects

*LUNG cancer & genetics, *GENE expression, *NON-coding RNA, *CANCER cell proliferation, *RETINOBLASTOMA protein

Abstract

Maternally expressed gene 3 (MEG3, mouse homolog Gtl2) encodes a long noncoding RNA (lncRNA) that is expressed in many normal tissues, but is suppressed in various cancer cell lines and tumors, suggesting it plays a functional role as a tumor suppressor. Hypermethylation has been shown to contribute to this loss of expression. We now demonstrate that MEG3 expression is regulated by the retinoblastoma protein (Rb) pathway and correlates with a change in cell proliferation. Microarray analysis of mouse embryonic fibroblasts (MEFs) isolated from mice with genetic deletion of all three Rb family members (TKO) revealed a significant silencing of Gtl2/MEG3 expression compared to WT MEFs, and re-expression of Gtl2/MEG3 caused decrease in cell proliferation and increased apoptosis. MEG3 levels also were suppressed in A549 lung cancer cells compared with normal human bronchial epithelial (NHBE) cells, and, similar to the TKO cells, re-constitution of MEG3 led to a decrease in cell proliferation and elevated apoptosis. Activation of pRb by treatment of A549 and SK-MES-1 cells with palbociclib, a CDK4/6 inhibitor, increased the expression of MEG3 in a dose-dependent manner, while knockdown of pRb/p107 attenuated this effect. In addition, expression of phosphorylation-deficient mutant of pRb increased MEG3 levels in both lung cancer cell types. Treatment of these cells with palbociclib also decreased the expression of pRb-regulated DNA methyltransferase 1 (DNMT1), while conversely, knockdown of DNMT1 resulted in increased expression of MEG3. As gene methylation has been suggested for MEG3 regulation, we found that palbociclib resulted in decreased methylation of the MEG3 locus similar to that observed with 5-aza-deoxycytidine. Anti-sense oligonucleotide silencing of drug-induced MEG3 expression in A549 and SK-MES-1 cells partially rescued the palbociclib-mediated decrease in cell proliferation, while analysis of the TCGA database revealed decreased MEG3 expression in human lung tumors harboring a disrupted RB pathway. Together, these data suggest that disruption of the pRb-DNMT1 pathway leads to a decrease in MEG3 expression, thereby contributing to the pro-proliferative state of certain cancer cells. [ABSTRACT FROM AUTHOR]

Published

2016

23. LapF and Its Regulation by Fis Affect the Cell Surface Hydrophobicity of Pseudomonas putida.

Author

Lahesaare, Andrio, Ainelo, Hanna, Teppo, Annika, Kivisaar, Maia, Heipieper, Hermann J., and Teras, Riho

Subjects

*PSEUDOMONAS putida, *BACTERIAL adaptation, *BACTERIAL antigens, *CELL surface antigens, *MOLECULAR cloning

Abstract

The ability of bacteria to regulate cell surface hydrophobicity is important for the adaptation to different environmental conditions. The hydrophobicity of cell surface can be determined by several factors, including outer membrane and surface proteins. In this study, we report that an adhesin LapF influences cell surface hydrophobicity of Pseudomonas putida. Cells lacking LapF are less hydrophobic than wild-type cells in stationary growth phase. Moreover, the overexpression of the global regulator Fis decreases surface hydrophobicity by repressing the expression of lapF. Flow cytometry analysis revealed that bacteria producing LapF are more viable when confronted with methanol (a hydrophilic compound) but are more susceptible to 1-octanol (a hydrophobic compound). Thus, these results revealed that LapF is the hydrophobicity factor for the cell surface of P. putida. [ABSTRACT FROM AUTHOR]

Published

2016

24. Step-Wise Increase in Tigecycline Resistance in Klebsiella pneumoniae Associated with Mutations in ramR, lon and rpsJ.

Author

Fang, Li, Chen, Qiong, Shi, Keren, Li, Xi, Shi, Qiucheng, He, Fang, Zhou, Jiancang, Yu, Yunsong, and Hua, Xiaoting

Subjects

*MULTIDRUG resistance in bacteria, *KLEBSIELLA pneumoniae, *GENETIC mutation, *PNEUMONIA treatment, *URINARY tract infection treatment, *DISEASE complications, *TIGECYCLINE

Abstract

Klebsiella pneumoniae is a gram-negative bacterium that causes numerous diseases, including pneumonia and urinary tract infections. An increase in multidrug resistance has complicated the treatment of these bacterial infections, and although tigecycline shows activity against a broad spectrum of bacteria, resistant strains have emerged. In this study, the whole genomes of two clinical and six laboratory-evolved strains were sequenced to identify putative mutations related to tigecycline resistance. Of seven tigecycline-resistant strains, seven (100%) had ramR mutations, five (71.4%) had lon mutations, one (14.2%) had a ramA mutation, and one (14.2%) had an rpsJ mutation. A higher fitness cost was observed in the laboratory-evolved strains but not in the clinical strains. A transcriptome analysis demonstrated high expression of the ramR operon and acrA in all tigecycline-resistant strains. Genes involved in nitrogen metabolism were induced in the laboratory-evolved strains compared with the wild-type and clinical strains, and this difference in nitrogen metabolism reflected the variation between the laboratory-evolved and the clinical strains. Complementation experiments showed that both the wild-type ramR and the lon genes could partially restore the tigecycline sensitivity of K. pneumoniae. We believe that this manuscript describes the first construct of a lon mutant in K. pneumoniae, which allowed confirmation of its association with tigecycline resistance. Our findings illustrate the importance of the ramR operon and the lon and rpsJ genes in K. pneumoniae resistance to tigecycline. [ABSTRACT FROM AUTHOR]

Published

2016

25. The Phospholipid:Diacylglycerol Acyltransferase Lro1 Is Responsible for Hepatitis C Virus Core-Induced Lipid Droplet Formation in a Yeast Model System.

Author

Iwasa, Shingo, Sato, Naoko, Wang, Chao-Wen, Cheng, Yun-Hsin, Irokawa, Hayato, Hwang, Gi-Wook, Naganuma, Akira, and Kuge, Shusuke

Subjects

*PHOSPHOLIPIDS, *DIGLYCERIDES, *ACYLTRANSFERASES, *CHRONIC hepatitis C, *YEAST, *FATTY degeneration

Abstract

Chronic infection with the hepatitis C virus frequently induces steatosis, which is a significant risk factor for liver pathogenesis. Steatosis is characterized by the accumulation of lipid droplets in hepatocytes. The structural protein core of the virus induces lipid droplet formation and localizes on the surface of the lipid droplets. However, the precise molecular mechanisms for the core-induced formation of lipid droplets remain elusive. Recently, we showed that the expression of the core protein in yeast as a model system could induce lipid droplet formation. In this study, we probed the cellular factors responsible for the formation of core-induced lipid-droplets in yeast cells. We demonstrated that one of the enzymes responsible for triglyceride synthesis, a phospholipid:diacylglycerol acyltransferase (Lro1), is required for the core-induced lipid droplet formation. While core proteins inhibit Lro1 degradation and alter Lro1 localization, the characteristic localization of Lro1 adjacent to the lipid droplets appeared to be responsible for the core-induced lipid droplet formation. RNA virus genomes have evolved using high mutation rates to maintain their ability to replicate. Our observations suggest a functional relationship between the core protein with hepatocytes and yeast cells. The possible interactions between core proteins and the endoplasmic reticulum membrane affect the mobilization of specific proteins. [ABSTRACT FROM AUTHOR]

Published

2016

26. Production of 3-Hydroxypropionic Acid via the Propionyl-CoA Pathway Using Recombinant Escherichia coli Strains.

Author

Luo, Hui, Zhou, Dafeng, Liu, Xiaohui, Nie, Zhihua, Quiroga-Sánchez, Diego Leandro, and Chang, Yanhong

Subjects

*PROPIONATES, *ESCHERICHIA coli, *METABOLISM, *CHLOROFLEXUS aurantiacus, *CELL culture

Abstract

Our study aimed to produce the commercially promising platform chemical 3-hydroxypropionic acid (3-HP) via the propionyl-CoA pathway in genetically engineered Escherichia coli. Recombinant E. coli Ec-P overexpressing propionyl-CoA dehydrogenase (PACD, encoded by the pacd gene from Candida rugosa) under the T7 promoter produced 1.33 mM of 3-HP in a shake flask culture supplemented with 0.5% propionate. When propionate CoA-transferase (PCT, encoded by the pct gene from Megasphaera elsdenii) and 3-hydroxypropionyl-CoA dehydratase (HPCD, encoded by the hpcd gene from Chloroflexus aurantiacus) were expressed along with PACD, the 3-HP titer of the resulting E. coli Ec-PPH strain was improved by 6-fold. The effect of the cultivation conditions on the 3-HP yield from propionate in the Ec-PPH strain was also investigated. When cultured at 30°C with 1% glucose in addition to propionate, 3-HP production by Ec-PPH increased 2-fold and 12-fold compared to the cultivation at 37°C (4.23 mM) or without glucose (0.68 mM). Deletion of the ygfH gene encoding propionyl-CoA: succinate CoA-transferase from Ec-PPH (resulting in the strain Ec-△Y-PPH) led to increase of 3-HP production in shake flask experiments (15.04 mM), whereas the strain Ec-△Y-PPH with deletion of the prpC gene (encoding methylcitrate synthase in the methylcitrate cycle) produced 17.76 mM of 3-HP. The strain Ec-△Y-△P-PPH with both ygfH and prpC genes deleted produced 24.14 mM of 3-HP, thus showing an 18-fold increase in the 3-HP titer in compare to the strain Ec-P. [ABSTRACT FROM AUTHOR]

Published

2016

27. Epitope-Tagged Autotransporters as Single-Cell Reporters for Gene Expression by a Salmonella Typhimurium wbaP Mutant.

Author

Curkić, Ismeta, Schütz, Monika, Oberhettinger, Philipp, Diard, Médéric, Claassen, Manfred, Linke, Dirk, and Hardt, Wolf-Dietrich

Subjects

*EPITOPES, *GENE expression, *SALMONELLA typhimurium, *PHENOTYPES, *BACTERIAL population, *FLUOROPHORES

Abstract

Phenotypic diversity is an important trait of bacterial populations and can enhance fitness of the existing genotype in a given environment. To characterize different subpopulations, several studies have analyzed differential gene expression using fluorescent reporters. These studies visualized either single or multiple genes within single cells using different fluorescent proteins. However, variable maturation and folding kinetics of different fluorophores complicate the study of dynamics of gene expression. Here, we present a proof-of-principle study for an alternative gene expression system in a wbaP mutant of Salmonella Typhimurium (S. Tm) lacking the O-sidechain of the lipopolysaccharide. We employed the hemagglutinin (HA)-tagged inverse autotransporter invasin (invAHA) as a transcriptional reporter for the expression of the type three secretion system 1 (T1) in S. Tm. Using a two-reporter approach with GFP and the InvAHA in single cells, we verify that this reporter system can be used for T1 gene expression analysis, at least in strains lacking the O-antigen (wbaP), which are permissive for detection of the surface-exposed HA-epitope. When we placed the two reporters gfp and invAHA under the control of either one or two different promoters of the T1 regulon, we were able to show correlative expression of both reporters. We conclude that the invAHA reporter system is a suitable tool to analyze T1gene expression in S. Tm and propose its applicability as molecular tool for gene expression studies within single cells. [ABSTRACT FROM AUTHOR]

Published

2016

28. The Staphylococcus aureus Global Regulator MgrA Modulates Clumping and Virulence by Controlling Surface Protein Expression.

Author

Crosby, Heidi A., Schlievert, Patrick M., Merriman, Joseph A., King, Jessica M., Salgado-Pabón, Wilmara, and Horswill, Alexander R.

Subjects

*STAPHYLOCOCCUS aureus, *PROTEIN expression, *MICROBIAL virulence, *RNA sequencing, *FIBRINOGEN

Abstract

Staphylococcus aureus is a human commensal and opportunistic pathogen that causes devastating infections in a wide range of locations within the body. One of the defining characteristics of S. aureus is its ability to form clumps in the presence of soluble fibrinogen, which likely has a protective benefit and facilitates adhesion to host tissue. We have previously shown that the ArlRS two-component regulatory system controls clumping, in part by repressing production of the large surface protein Ebh. In this work we show that ArlRS does not directly regulate Ebh, but instead ArlRS activates expression of the global regulator MgrA. Strains lacking mgrA fail to clump in the presence of fibrinogen, and clumping can be restored to an arlRS mutant by overexpressing either arlRS or mgrA, indicating that ArlRS and MgrA constitute a regulatory pathway. We used RNA-seq to show that MgrA represses ebh, as well as seven cell wall-associated proteins (SraP, Spa, FnbB, SasG, SasC, FmtB, and SdrD). EMSA analysis showed that MgrA directly represses expression of ebh and sraP. Clumping can be restored to an mgrA mutant by deleting the genes for Ebh, SraP and SasG, suggesting that increased expression of these proteins blocks clumping by steric hindrance. We show that mgrA mutants are less virulent in a rabbit model of endocarditis, and virulence can be partially restored by deleting the genes for the surface proteins ebh, sraP, and sasG. While mgrA mutants are unable to clump, they are known to have enhanced biofilm capacity. We demonstrate that this increase in biofilm formation is partially due to up-regulation of SasG, a surface protein known to promote intercellular interactions. These results confirm that ArlRS and MgrA constitute a regulatory cascade, and that they control expression of a number of genes important for virulence, including those for eight large surface proteins. [ABSTRACT FROM AUTHOR]

Published

2016

29. Enhanced snoMEN Vectors Facilitate Establishment of GFP–HIF-1α Protein Replacement Human Cell Lines.

Author

Ono, Motoharu, Yamada, Kayo, Bensaddek, Dalila, Afzal, Vackar, Biddlestone, John, Ortmann, Brian, Mudie, Sharon, Boivin, Vincent, Scott, Michelle S., Rocha, Sonia, and Lamond, Angus I.

Subjects

*GENETIC vectors, *GREEN fluorescent protein, *CELL analysis, *NUCLEOTIDE sequence, *GENE therapy, *CHIMERIC proteins, *MASS spectrometry

Abstract

The snoMEN (RNA odulator of gene xpressio) vector technology was developed from a human box C/D snoRNA, HBII-180C, which contains an internal sequence that can be manipulated to make it complementary to RNA targets, allowing knock-down of targeted genes. Here we have screened additional human nucleolar snoRNAs and assessed their application for gene specific knock-downs to improve the efficiency of snoMEN vectors. We identify and characterise a new snoMEN vector, termed 47snoMEN, that is derived from box C/D snoRNA U47, demonstrating its use for knock-down of both endogenous cellular proteins and G/YFP-fusion proteins. Using multiplex 47snoMEM vectors that co-express multiple 47snoMEN in a single transcript, each of which can target different sites in the same mRNA, we document >3-fold increase in knock-down efficiency when compared with the original HBII-180C based snoMEN. The multiplex 47snoMEM vector allowed the construction of human protein replacement cell lines with improved efficiency, including the establishment of novel GFP–HIF-1α replacement cells. Quantitative mass spectrometry analysis confirmed the enhanced efficiency and specificity of protein replacement using the 47snoMEN-PR vectors. The 47snoMEN vectors expand the potential applications for snoMEN technology in gene expression studies, target validation and gene therapy. [ABSTRACT FROM AUTHOR]

Published

2016

30. A Novel Manno-Oligosaccharide Binding Protein Identified in Alkaliphilic Bacillus sp. N16-5 Is Involved in Mannan Utilization.

Author

Song, Yajian, Li, Jinshan, Meng, Shan, Yin, Liang, Xue, Yanfen, and Ma, Yanhe

Subjects

*OLIGOSACCHARIDES, *CARRIER proteins, *BACILLUS (Bacteria), *MANNANS, *CHEMICAL affinity, *ISOTHERMAL titration calorimetry

Abstract

ManH, a novel substrate-binding protein of an ABC transporter, was identified from the mannan utilization gene cluster of Bacillus sp. N16-5. We cloned, overexpressed, and purified ManH and measured its binding affinity to different substrates by isothermal titration calorimetry. ManH binds to mannotriose, mannotetraose, mannopentose, and galactosyl-mannotriose with dissociation constants in the micromolar range. Deletion of manH led to decreased growth ability of the strain when cultivated in medium with manno-oligosaccharides or mannan as the carbon source. ManH belongs to a manno-oligosaccharide transporter and plays an important role in mannan utilization by Bacillus sp. N16-5. [ABSTRACT FROM AUTHOR]

Published

2016

31. A Fast and Practical Yeast Transformation Method Mediated by Escherichia coli Based on a Trans-Kingdom Conjugal Transfer System: Just Mix Two Cultures and Wait One Hour.

Author

Moriguchi, Kazuki, Yamamoto, Shinji, Ohmine, Yuta, and Suzuki, Katsunori

Subjects

*ESCHERICHIA coli, *DNA analysis, *CELL culture, *GENETIC vectors, *SACCHAROMYCES

Abstract

Trans-kingdom conjugation is a phenomenon by which DNA is transferred into a eukaryotic cell by a bacterial conjugal transfer system. Improvement in this method to facilitate the rapid co-cultivation of donor bacterial and recipient eukaryotic cell cultures could make it the simplest transformation method, requiring neither isolation of vector DNA nor preparation of competent recipient cells. To evaluate this potential advantage of trans-kingdom conjugation, we examined this simple transformation method using vector combinations, helper plasmids, and recipient Saccharomyces cerevisiae strains. Mixing donor Escherichia coli and recipient S. cerevisiae overnight cultures (50 μL each) consistently yielded on the order of 101 transformants using the popular experimental strain BY4742 derived from S288c and a shuttle vector for trans-kingdom conjugation. Transformation efficiency increased to the order of 102 using a high receptivity trans-kingdom conjugation strain. In addition, either increasing the amount of donor cells or pretreating the recipient cells with thiols such as dithiothreitol improved the transformation efficiency by one order of magnitude. This simple trans-kingdom conjugation-mediated transformation method could be used as a practical yeast transformation method upon enrichment of available vectors and donor E. coli strains. [ABSTRACT FROM AUTHOR]

Published

2016

32. A Vector with a Single Promoter for In Vitro Transcription and Mammalian Cell Expression of CRISPR gRNAs.

Author

Romanienko, Peter J., Giacalone, Joseph, Ingenito, Joanne, Wang, Yijie, Isaka, Mayumi, Johnson, Thomas, You, Yun, and Mark, Willie H.

Subjects

*PROMOTERS (Genetics), *IN vitro studies, *RNA analysis, *PROTEIN expression, *MICROINJECTIONS

Abstract

The genomes of more than 50 organisms have now been manipulated due to rapid advancement of gene editing technology. One way to perform gene editing in the mouse using the CRISPR/CAS system, guide RNA (gRNA) and CAS9 mRNA transcribed in vitro are microinjected into fertilized eggs that are then allowed to develop to term. As a rule, gRNAs are tested first in tissue culture cells and the one with the highest locus-specific cleavage activity is chosen for microinjection. For cell transfections, gRNAs are typically expressed using the human U6 promoter (hU6). However, gRNAs for microinjection into zygotes are obtained by in vitro transcription from a T7 bacteriophage promoter in a separate plasmid vector. Here, we describe the design and construction of a combined U6T7 hybrid promoter from which the same gRNA sequence can be expressed. An expression vector containing such a hybrid promoter can now be used to generate gRNA for testing in mammalian cells as well as for microinjection purposes. The gRNAs expressed and transcribed from this vector are found to be functional in cells as well as in mice. [ABSTRACT FROM AUTHOR]

Published

2016

33. Biological Activity of the Alternative Promoters of the Dictyostelium discoideum Adenylyl Cyclase A Gene.

Author

Rodriguez-Centeno, Javier and Sastre, Leandro

Subjects

*DICTYOSTELIUM discoideum, *PROMOTERS (Genetics), *ADENYLATE cyclase, *FUNGAL genes, *FRUITING bodies (Fungi), *STARVATION, *FUNGI

Abstract

Amoebae of the Dictyostelium discoideum species form multicellular fruiting bodies upon starvation. Cyclic adenosine monophosphate (cAMP) is used as intercellular signalling molecule in cell-aggregation, cell differentiation and morphogenesis. This molecule is synthesized by three adenylyl cyclases, one of which, ACA, is required for cell aggregation. The gene coding for ACA (acaA) is transcribed from three different promoters that are active at different developmental stages. Promoter 1 is active during cell-aggregation, promoters 2 and 3 are active in prespore and prestalk tip cells at subsequent developmental stages. The biological relevance of acaA expression from each of the promoters has been studied in this article. The acaA gene was expressed in acaA-mutant cells, that do not aggregate, under control of each of the three acaA promoters. acaA expression under promoter 1 control induced cell aggregation although subsequent development was delayed, very small fruiting bodies were formed and cell differentiation genes were expressed at very low levels. Promoter 2-driven acaA expression induced the formation of small aggregates and small fruiting bodies were formed at the same time as in wild-type strains and differentiation genes were also expressed at lower levels. Expression of acaA from promoter 3 induced aggregates and fruiting bodies formation and their size and the expression of differentiation genes were more similar to that of wild-type cells. Expression of acaA from promoters 1 and 2 in AX4 cells also produced smaller structures. In conclusion, the expression of acaA under control of the aggregation-specific Promoter 1 is able to induce cell aggregation in acaA-mutant strains. Expression from promoters 2 and 3 also recovered aggregation and development although promoter 3 induced a more complete recovery of fruiting body formation. [ABSTRACT FROM AUTHOR]

Published

2016

34. A simple method for ex vivo honey bee cell culture capable of in vitro gene expression analysis

Author

Takumi Kayukawa, Mikio Yoshiyama, Kiyoshi Kimura, Gaku Akiduki, Kazuyo Watanabe, Kakeru Yokoi, Masatsugu Hatakeyama, and Hiroko Hoshida

Subjects

Hemocytes, Molecular biology, Cell Culture Techniques, Gene Expression, Biochemistry, Green fluorescent protein, White Blood Cells, RNA interference, Animal Cells, Gene expression, Medicine and Health Sciences, Cells, Cultured, Plasmid Vectors, Multidisciplinary, Expression vector, Eukaryota, Transfection, Bees, Cell biology, Insects, Nucleic acids, Genetic interference, Medicine, Engineering and Technology, Epigenetics, Biological Cultures, Cellular Types, Honey Bees, Genetic Engineering, Plasmids, Research Article, Biotechnology, animal structures, Arthropoda, Science, Immune Cells, Green Fluorescent Proteins, Immunology, Bioengineering, Biology, DNA construction, Research and Analysis Methods, Genetics, Animals, Molecular Biology Techniques, Blood Cells, Biology and life sciences, Gene Expression Profiling, fungi, Organisms, Honey bee, Cell Biology, Cell Cultures, Hymenoptera, Invertebrates, Culture Media, Gene Expression Regulation, Cell culture, Plasmid Construction, RNA, Zoology, Entomology, Ex vivo

Abstract

Cultured cells are a very powerful tool for investigating biological events in vitro; therefore, cell lines have been established not only in model insect species, but also in non-model species. However, there are few reports on the establishment of stable cell lines and development of systems to introduce genes into the cultured cells of the honey bee (Apis mellifera). We describe a simple ex vivo cell culture system for the honey bee. Hemocyte cells obtained from third and fourth instar larvae were cultured in commercial Grace’s insect medium or MGM-450 insect medium for more than two weeks maintaining a normal morphology without deterioration. After an expression plasmid vector bearing the enhanced green fluorescent protein (egfp) gene driven by the immediate early 2 (IE2) viral promoter was transfected into cells, EGFP fluorescence was detected in cells for more than one week from one day after transfection. Furthermore, double-stranded RNA corresponding to a part of the egfp gene was successfully introduced into cells and interfered with egfp gene expression. A convenient and reproducible method for an ex vivo cell culture that is fully practicable for gene expression assays was established for the honey bee.

Published

2021

35. Vaccines against Botulism

Author

Grace Sundeen and Joseph T. Barbieri

Subjects

botulism, botulinum neurotoxins, vaccines, plasmid vectors, viral vectors, toxoids, genetically inactivated toxoids, Medicine

Abstract

Botulinum neurotoxins (BoNT) cause the flaccid paralysis of botulism by inhibiting the release of acetylcholine from motor neurons. There are seven serotypes of BoNT (A-G), with limited therapies, and no FDA approved vaccine for botulism. An investigational formalin-inactivated penta-serotype-BoNT/A-E toxoid vaccine was used to vaccinate people who are at high risk of contracting botulism. However, this formalin-inactivated penta-serotype-BoNT/A-E toxoid vaccine was losing potency and was discontinued. This article reviews the different vaccines being developed to replace the discontinued toxoid vaccine. These vaccines include DNA-based, viral vector-based, and recombinant protein-based vaccines. DNA-based vaccines include plasmids or viral vectors containing the gene encoding one of the BoNT heavy chain receptor binding domains (HC). Viral vectors reviewed are adenovirus, influenza virus, rabies virus, Semliki Forest virus, and Venezuelan Equine Encephalitis virus. Among the potential recombinant protein vaccines reviewed are HC, light chain-heavy chain translocation domain, and chemically or genetically inactivated holotoxin.

Published

2017

36. Construction of the recombinant broad-host-range plasmids providing their bacterial hosts arsenic resistance and arsenite oxidation ability.

Author

Drewniak, Lukasz, Ciezkowska, Martyna, Radlinska, Monika, and Sklodowska, Aleksandra

Subjects

*PLASMIDS, *HOSTS (Biology), *BACTERIAL population, *ARSENITES, *PHENOTYPES, *PROTEOBACTERIA

Abstract

The plasmid pSinA of Sinorhizobium sp. M14 was used as a source of functional phenotypic modules, encoding proteins involved in arsenite oxidation and arsenic resistance, to obtain recombinant broad-host-range plasmids providing their bacterial hosts arsenic resistance and arsenite oxidative ability. An arsenite oxidation module was cloned into pBBR1MCS-2 vector yielding plasmid vector pAIO1, while an arsenic resistance module was cloned into pCM62 vector yielding plasmid pARS1. Both plasmid constructs were introduced (separately and together) into the cells of phylogenetically distant (representing Alpha -, Beta -, and Gammaproteobacteria ) and physiologically diversified (unable to oxidize arsenite and susceptible/resistant to arsenite and arsenate) bacteria. Functional analysis of the modified strains showed that: (i) the plasmid pARS1 can be used for the construction of strains with an increased resistance to arsenite [up to 20 mM of As(III), (ii) the presence of the plasmid pAIO1 in bacteria previously unable to oxidize As(III) to As(V), contributes to the acquisition of arsenite oxidation abilities by these cells, (iii) the highest arsenite utilization rate are observed in the culture of strains harbouring both the plasmids pAIO1 and pARS1, (iv) the strains harbouring the plasmid pAIO1 were able to grow on arsenic-contaminated mine waters (∼3.0 mg As L −1 ) without any supplementation. [ABSTRACT FROM AUTHOR]

Published

2015

37. Novel Expression Vectors Enabling Induction of Gene Expression by Small-Interfering RNAs and MicroRNAs.

Author

Harel, Liraz, Gefen, Nir, Carmi, Ofira, Orbach, Pini, Einat, Paz, and Abitbol, Guy

Subjects

*CANCER treatment, *GENE therapy, *GENE expression, *SMALL interfering RNA, *MICRORNA genetics, *MOLECULAR biology, *EUKARYOTES

Abstract

Small-interfering RNAs and microRNAs are small ∼21–22 nucleotide long RNAs capable of posttranscriptional suppression of gene expression. The synthetic siRNAs are especially designed to target pre-specified genes and are common molecular biology tools. The miRNAs are endogenous regulators of gene expression found in a wide variety of eukaryotes. miRNAs are currently utilized for diagnostics applications. Therapeutically, various miRNA-antagonizing tools are being explored and miRNAs are also utilized for cell-specific inhibition of the expression of gene therapy vectors harboring target sites for specific miRNAs. Here we show, for the first time, that siRNAs and miRNAs can be harnessed to induce gene expression. We designed special expression vectors in which target sites for artificial siRNAs or endogenous miRNAs are located between the transgene and an Upstream Inhibitory Region (UIR). We hypothesized that cleavage of the mRNA by siRNAs or miRNAs will separate the transgene from the UIR and the resulting uncapped mRNA will be capable of being translated. A UIR composed of seven open reading frames was found to be the most efficient inhibitor of the translation of the downstream transgene. We show that under such a configuration both artificial siRNAs and endogenous miRNAs were capable of inducing transgene expression. We show that using the diphtheria toxin A-chain gene, in combination with target sites for highly expressed miRNAs, specific induction of cell-death can be achieved, setting the stage for application to cancer therapy. [ABSTRACT FROM AUTHOR]

Published

2014

38. Co-Cultivation of Fungal and Microalgal Cells as an Efficient System for Harvesting Microalgal Cells, Lipid Production and Wastewater Treatment.

Author

Wrede, Digby, Taha, Mohamed, Miranda, Ana F., Kadali, Krishna, Stevenson, Trevor, Ball, Andrew S., and Mouradov, Aidyn

Subjects

*WASTEWATER treatment, *MICROALGAE, *LIPIDS, *FLOCCULATION, *AGRICULTURAL biotechnology, *PLANT genes

Abstract

The challenges which the large scale microalgal industry is facing are associated with the high cost of key operations such as harvesting, nutrient supply and oil extraction. The high-energy input for harvesting makes current commercial microalgal biodiesel production economically unfeasible and can account for up to 50% of the total cost of biofuel production. Co-cultivation of fungal and microalgal cells is getting increasing attention because of high efficiency of bio-flocculation of microalgal cells with no requirement for added chemicals and low energy inputs. Moreover, some fungal and microalgal strains are well known for their exceptional ability to purify wastewater, generating biomass that represents a renewable and sustainable feedstock for biofuel production. We have screened the flocculation efficiency of the filamentous fungus A. fumigatus against 11 microalgae representing freshwater, marine, small (5 µm), large (over 300 µm), heterotrophic, photoautotrophic, motile and non-motile strains. Some of the strains are commercially used for biofuel production. Lipid production and composition were analysed in fungal-algal pellets grown on media containing alternative carbon, nitrogen and phosphorus sources contained in wheat straw and swine wastewater, respectively. Co-cultivation of algae and A. fumigatus cells showed additive and synergistic effects on biomass production, lipid yield and wastewater bioremediation efficiency. Analysis of fungal-algal pellet's fatty acids composition suggested that it can be tailored and optimised through co-cultivating different algae and fungi without the need for genetic modification. [ABSTRACT FROM AUTHOR]

Published

2014

39. Genomic Analysis of Sleeping Beauty Transposon Integration in Human Somatic Cells.

Author

Turchiano, Giandomenico, Latella, Maria Carmela, Gogol-Döring, Andreas, Cattoglio, Claudia, Mavilio, Fulvio, Izsvák, Zsuzsanna, Ivics, Zoltán, and Recchia, Alessandra

Subjects

*TRANSPOSONS, *SOMATIC cells, *FUNCTIONAL genomics, *GENETIC transformation, *TRANSPOSASES, *KERATINOCYTES

Abstract

The Sleeping Beauty (SB) transposon is a non-viral integrating vector system with proven efficacy for gene transfer and functional genomics. However, integration efficiency is negatively affected by the length of the transposon. To optimize the SB transposon machinery, the inverted repeats and the transposase gene underwent several modifications, resulting in the generation of the hyperactive SB100X transposase and of the high-capacity “sandwich” (SA) transposon. In this study, we report a side-by-side comparison of the SA and the widely used T2 arrangement of transposon vectors carrying increasing DNA cargoes, up to 18 kb. Clonal analysis of SA integrants in human epithelial cells and in immortalized keratinocytes demonstrates stability and integrity of the transposon independently from the cargo size and copy number-dependent expression of the cargo cassette. A genome-wide analysis of unambiguously mapped SA integrations in keratinocytes showed an almost random distribution, with an overrepresentation in repetitive elements (satellite, LINE and small RNAs) compared to a library representing insertions of the first-generation transposon vector and to gammaretroviral and lentiviral libraries. The SA transposon/SB100X integrating system therefore shows important features as a system for delivering large gene constructs for gene therapy applications. [ABSTRACT FROM AUTHOR]

Published

2014

40. New Developments of RNAi in Paracoccidioides brasiliensis: Prospects for High-Throughput, Genome-Wide, Functional Genomics.

Author

Goes, Tercio, Bailão, Elisa Flavia L. C., Correa, Cristiane R., Bozzi, Adriana, Santos, Luara I., Gomes, Dawidson A., Soares, Celia M. A., and Goes, Alfredo M.

Subjects

*PARACOCCIDIOIDES brasiliensis, *RNA interference, *FUNGAL genetics, *GENOMES, *GENOMICS, *AGROBACTERIUM tumefaciens, *BLEOMYCIN

Abstract

Background: The Fungal Genome Initiative of the Broad Institute, in partnership with the Paracoccidioides research community, has recently sequenced the genome of representative isolates of this human-pathogen dimorphic fungus: Pb18 (S1), Pb03 (PS2) and Pb01. The accomplishment of future high-throughput, genome-wide, functional genomics will rely upon appropriate molecular tools and straightforward techniques to streamline the generation of stable loss-of-function phenotypes. In the past decades, RNAi has emerged as the most robust genetic technique to modulate or to suppress gene expression in diverse eukaryotes, including fungi. These molecular tools and techniques, adapted for RNAi, were up until now unavailable for P. brasiliensis. Methodology/Principal Findings: In this paper, we report Agrobacterium tumefaciens mediated transformation of yeast cells for high-throughput applications with which higher transformation frequencies of 150±24 yeast cell transformants per 1×106 viable yeast cells were obtained. Our approach is based on a bifunctional selective marker fusion protein consisted of the Streptoalloteichus hindustanus bleomycin-resistance gene (Shble) and the intrinsically fluorescent monomeric protein mCherry which was codon-optimized for heterologous expression in P. brasiliensis. We also report successful GP43 gene knock-down through the expression of intron-containing hairpin RNA (ihpRNA) from a Gateway-adapted cassette (cALf) which was purpose-built for gene silencing in a high-throughput manner. Gp43 transcript levels were reduced by 73.1±22.9% with this approach. Conclusions/Significance: We have a firm conviction that the genetic transformation technique and the molecular tools herein described will have a relevant contribution in future Paracoccidioides spp. functional genomics research. [ABSTRACT FROM AUTHOR]

Published

2014

41. Cyanobacterial Light-Driven Proton Pump, Gloeobacter Rhodopsin: Complementarity between Rhodopsin-Based Energy Production and Photosynthesis.

Author

Choi, Ah Reum, Shi, Lichi, Brown, Leonid S., and Jung, Kwang-Hwan

Subjects

*CYANOBACTERIAL genes, *PROTON pump inhibitors, *RHODOPSIN, *PHYCOBILISOMES, *THYLAKOIDS, *TRANSDUCERS, *AMINO acid sequence, *GENE expression in bacteria

Abstract

A homologue of type I rhodopsin was found in the unicellular Gloeobacter violaceus PCC7421, which is believed to be primitive because of the lack of thylakoids and peculiar morphology of phycobilisomes. The Gloeobacter rhodopsin (GR) gene encodes a polypeptide of 298 amino acids. This gene is localized alone in the genome unlike cyanobacterium Anabaena opsin, which is clustered together with 14 kDa transducer gene. Amino acid sequence comparison of GR with other type I rhodopsin shows several conserved residues important for retinal binding and H+ pumping. In this study, the gene was expressed in Escherichia coli and bound all-trans retinal to form a pigment (λmax  = 544 nm at pH 7). The pKa of proton acceptor (Asp121) for the Schiff base, is approximately 5.9, so GR can translocate H+ under physiological conditions (pH 7.4). In order to prove the functional activity in the cell, pumping activity was measured in the sphaeroplast membranes of E. coli and one of Gloeobacter whole cell. The efficient proton pumping and rapid photocycle of GR strongly suggests that Gloeobacter rhodopsin functions as a proton pumping in its natural environment, probably compensating the shortage of energy generated by chlorophyll-based photosynthesis without thylakoids. [ABSTRACT FROM AUTHOR]

Published

2014

42. A Novel System for Simultaneous or Sequential Integration of Multiple Gene-Loading Vectors into a Defined Site of a Human Artificial Chromosome.

Author

Suzuki, Teruhiko, Kazuki, Yasuhiro, Oshimura, Mitsuo, and Hara, Takahiko

Subjects

*GENETIC vectors, *RECOMBINANT DNA, *MAMMALIAN cell cycle, *ARTIFICIAL chromosomes, *BIOMEDICAL engineering

Abstract

Human artificial chromosomes (HACs) are gene-delivery vectors suitable for introducing large DNA fragments into mammalian cells. Although a HAC theoretically incorporates multiple gene expression cassettes of unlimited DNA size, its application has been limited because the conventional gene-loading system accepts only one gene-loading vector (GLV) into a HAC. We report a novel method for the simultaneous or sequential integration of multiple GLVs into a HAC vector (designated as the SIM system) via combined usage of Cre, FLP, Bxb1, and φC31 recombinase/integrase. As a proof of principle, we first attempted simultaneous integration of three GLVs encoding EGFP, Venus, and TdTomato into a gene-loading site of a HAC in CHO cells. These cells successfully expressed all three fluorescent proteins. Furthermore, microcell-mediated transfer of HACs enabled the expression of those fluorescent proteins in recipient cells. We next demonstrated that GLVs could be introduced into a HAC one-by-one via reciprocal usage of recombinase/integrase. Lastly, we introduced a fourth GLV into a HAC after simultaneous integration of three GLVs by FLP-mediated DNA recombination. The SIM system expands the applicability of HAC vectors and is useful for various biomedical studies, including cell reprogramming. [ABSTRACT FROM AUTHOR]

Published

2014

43. A Modular Cloning Toolbox for the Generation of Chloroplast Transformation Vectors.

Author

Vafaee, Yavar, Staniek, Agata, Mancheno-Solano, Maria, and Warzecha, Heribert

Subjects

*CLONING, *PLASTIDS, *CHLOROPLASTS, *GENETIC engineering, *ASEXUAL reproduction

Abstract

Plastid transformation is a powerful tool for basic research, but also for the generation of stable genetically engineered plants producing recombinant proteins at high levels or for metabolic engineering purposes. However, due to the genetic makeup of plastids and the distinct features of the transformation process, vector design, and the use of specific genetic elements, a large set of basic transformation vectors is required, making cloning a tedious and time-consuming effort. Here, we describe the adoption of standardized modular cloning (GoldenBraid) to the design and assembly of the full spectrum of plastid transformation vectors. The modular design of genetic elements allows straightforward and time-efficient build-up of transcriptional units as well as construction of vectors targeting any homologous recombination site of choice. In a three-level assembly process, we established a vector fostering gene expression and formation of griffithsin, a potential viral entry inhibitor and HIV prophylactic, in the plastids of tobacco. Successful transformation as well as transcript and protein production could be shown. In concert with the aforesaid endeavor, a set of modules facilitating plastid transformation was generated, thus augmenting the GoldenBraid toolbox. In short, the work presented in this study enables efficient application of synthetic biology methods to plastid transformation in plants. [ABSTRACT FROM AUTHOR]

Published

2014

44. Efficient Gene Targeting in Golden Syrian Hamsters by the CRISPR/Cas9 System.

Author

Fan, Zhiqiang, Li, Wei, Lee, Sang R., Meng, Qinggang, Shi, Bi, Bunch, Thomas D., White, Kenneth L., Kong, Il-Keun, and Wang, Zhongde

Subjects

*HAMSTERS, *GENE targeting, *CRISPRS, *NUCLEOTIDE sequence, *SOMATIC cells, *CYTOPLASM

Abstract

The golden Syrian hamster is the model of choice or the only rodent model for studying many human diseases. However, the lack of gene targeting tools in hamsters severely limits their use in biomedical research. Here, we report the first successful application of the CRISPR/Cas9 system to efficiently conduct gene targeting in hamsters. We designed five synthetic single-guide RNAs (sgRNAs)—three for targeting the coding sequences for different functional domains of the hamster STAT2 protein, one for KCNQ1, and one for PPP1R12C—and demonstrated that the CRISPR/Cas9 system is highly efficient in introducing site-specific mutations in hamster somatic cells. We then developed unique pronuclear (PN) and cytoplasmic injection protocols in hamsters and produced STAT2 knockout (KO) hamsters by injecting the sgRNA/Cas9, either in the form of plasmid or mRNA, targeting exon 4 of hamster STAT2. Among the produced hamsters, 14.3% and 88.9% harbored germline-transmitted STAT2 mutations from plasmid and mRNA injection, respectively. Notably, 10.4% of the animals produced from mRNA injection were biallelically targeted. This is the first success in conducting site-specific gene targeting in hamsters and can serve as the foundation for developing other genetically engineered hamster models for human disease. [ABSTRACT FROM AUTHOR]

Published

2014

45. Establishment of a Rabbit Oct4 Promoter-Based EGFP Reporter System.

Author

Quan, Longquan, Chen, Yongqiang, Song, Jun, Yan, Quanmei, Zhang, Quanjun, Lai, Sisi, Fan, Nana, Xin, Jige, Zou, Qingjian, and Lai, Liangxue

Subjects

*ANIMAL models in research, *RABBITS, *PHYLOGENY, *PLURIPOTENT stem cells, *TRANSCRIPTION factors, *FIBROBLASTS

Abstract

Rabbits are commonly used as laboratory animal models to investigate human diseases and phylogenetic development. However, pluripotent stem cells that contribute to germline transmission have yet to be established in rabbits. The transcription factor Oct4, also known as Pou5f1, is considered essential for the maintenance of the pluripotency of stem cells. Hence, pluripotent cells can be identified by monitoring Oct4 expression using a well-established Oct4 promoter-based reporter system. This study developed a rabbit Oct4 promoter-based enhanced green fluorescent protein (EGFP) reporter system by transfecting pROP2-EGFP into rabbit fetal fibroblasts (RFFs). The transgenic RFFs were used as donor cells for somatic cell nuclear transfer (SCNT). The EGFP expression was detected in the blastocysts and genital ridges of SCNT fetuses. Fibroblasts and neural stem cells (NSCs) were derived from the SCNT fetuses. EGFP was also reactivated in blastocysts after the second SCNT, and induced pluripotent stem cells (iPSCs) were obtained after reprogramming using Yamanaka's factors. The results above indicated that a rabbit reporter system used to monitor the differentiating status of cells was successfully developed. [ABSTRACT FROM AUTHOR]

Published

2014

46. Fitness Cost Implications of PhiC31-Mediated Site-Specific Integrations in Target-Site Strains of the Mexican Fruit Fly, Anastrepha ludens (Diptera: Tephritidae).

Author

Meza, José S., Díaz-Fleischer, Francisco, Sánchez-Velásquez, Lázaro R., Zepeda-Cisneros, Cristina Silvia, Handler, Alfred M., and Schetelig, Marc F.

Subjects

*SITE-specific mutagenesis, *TRANSGENES, *DNA, *ANASTREPHA, *DIPTERA, *PHYSIOLOGY

Abstract

Site-specific recombination technologies are powerful new tools for the manipulation of genomic DNA in insects that can improve transgenesis strategies such as targeting transgene insertions, allowing transgene cassette exchange and DNA mobilization for transgene stabilization. However, understanding the fitness cost implications of these manipulations for transgenic strain applications is critical. In this study independent piggyBac-mediated attP target-sites marked with DsRed were created in several genomic positions in the Mexican fruit fly, Anastrepha ludens. Two of these strains, one having an autosomal (attP_F7) and the other a Y-linked (attP_2-M6y) integration, exhibited fitness parameters (dynamic demography and sexual competitiveness) similar to wild type flies. These strains were thus selected for targeted insertion using, for the first time in mexfly, the phiC31-integrase recombination system to insert an additional EGFP-marked transgene to determine its effect on host strain fitness. Fitness tests showed that the integration event in the int_2-M6y recombinant strain had no significant effect, while the int_F7 recombinant strain exhibited significantly lower fitness relative to the original attP_F7 target-site host strain. These results indicate that while targeted transgene integrations can be achieved without an additional fitness cost, at some genomic positions insertion of additional DNA into a previously integrated transgene can have a significant negative effect. Thus, for targeted transgene insertions fitness costs must be evaluated both previous to and subsequent to new site-specific insertions in the target-site strain. [ABSTRACT FROM AUTHOR]

Published

2014

47. Analysis of the Role of Homology Arms in Gene-Targeting Vectors in Human Cells.

Author

Ishii, Ayako, Kurosawa, Aya, Saito, Shinta, and Adachi, Noritaka

Subjects

*SOMATIC cells, *GENE targeting, *DNA repair, *DNA ligases, *NUCLEOTIDE sequence, *BIOCHEMISTRY, *GENETIC engineering

Abstract

Random integration of targeting vectors into the genome is the primary obstacle in human somatic cell gene targeting. Non-homologous end-joining (NHEJ), a major pathway for repairing DNA double-strand breaks, is thought to be responsible for most random integration events; however, absence of DNA ligase IV (LIG4), the critical NHEJ ligase, does not significantly reduce random integration frequency of targeting vector in human cells, indicating robust integration events occurring via a LIG4-independent mechanism. To gain insights into the mechanism and robustness of LIG4-independent random integration, we employed various types of targeting vectors to examine their integration frequencies in LIG4-proficient and deficient human cell lines. We find that the integration frequency of targeting vector correlates well with the length of homology arms and with the amount of repetitive DNA sequences, especially SINEs, present in the arms. This correlation was prominent in LIG4-deficient cells, but was also seen in LIG4-proficient cells, thus providing evidence that LIG4-independent random integration occurs frequently even when NHEJ is functionally normal. Our results collectively suggest that random integration frequency of conventional targeting vectors is substantially influenced by homology arms, which typically harbor repetitive DNA sequences that serve to facilitate LIG4-independent random integration in human cells, regardless of the presence or absence of functional NHEJ. [ABSTRACT FROM AUTHOR]

Published

2014

48. Increased Drought Tolerance through the Suppression of ESKMO1 Gene and Overexpression of CBF-Related Genes in Arabidopsis.

Author

Xu, Fuhui, Liu, Zhixue, Xie, Hongyan, Zhu, Jian, Zhang, Juren, Kraus, Josef, Blaschnig, Tasja, Nehls, Reinhard, and Wang, Hong

Subjects

*DROUGHT tolerance, *GENE expression in plants, *ARABIDOPSIS, *SMALL interfering RNA, *VASCULAR system of plants, *PLANT morphogenesis, *AGRICULTURAL biotechnology

Abstract

Improved drought tolerance is always a highly desired trait for agricultural plants. Significantly increased drought tolerance in Arabidopsis thaliana (Columbia-0) has been achieved in our work through the suppression of ESKMO1 (ESK1) gene expression with small-interfering RNA (siRNA) and overexpression of CBF genes with constitutive gene expression. ESK1 has been identified as a gene linked to normal development of the plant vascular system, which is assumed directly related to plant drought response. By using siRNA that specifically targets ESK1, the gene expression has been reduced and drought tolerance of the plant has been enhanced dramatically in the work. However, the plant response to external abscisic acid application has not been changed. ICE1, CBF1, and CBF3 are genes involved in a well-characterized plant stress response pathway, overexpression of them in the plant has demonstrated capable to increase drought tolerance. By overexpression of these genes combining together with suppression of ESK1 gene, the significant increase of plant drought tolerance has been achieved in comparison to single gene manipulation, although the effect is not in an additive way. Accompanying the increase of drought tolerance via suppression of ESK1 gene expression, the negative effect has been observed in seeds yield of transgenic plants in normal watering conditions comparing with wide type plant. [ABSTRACT FROM AUTHOR]

Published

2014

49. Generation of Ugt1-Deficient Murine Liver Cell Lines Using TALEN Technology.

Author

Porro, Fabiola, Bockor, Luka, De Caneva, Alessia, Bortolussi, Giulia, and Muro, Andrés F.

Subjects

*CRIGLER-Najjar syndrome, *LIVER cells, *GENETIC disorders, *DNA restriction enzymes, *FRAMESHIFT mutation, *MISSENSE mutation

Abstract

The Crigler-Najjar Syndrome Type I (CNSI) is a rare genetic disorder caused by mutations in the Ugt1a1 gene. It is characterized by unconjugated hyperbilirubinemia that may result in severe neurologic damage and death if untreated. To date, liver transplantation is the only curative treatment. With the aim of generating mutant cell lines of the Ugt1 gene, we utilized the TALEN technology to introduce site-specific mutations in Ugt1 exon 4. We report a fast and efficient method to perform gene knockout in tissue culture cells, based on the use of TALEN pairs targeting restriction enzyme (RE) sites in the region of interest. This strategy overcame the presence of allele-specific single nucleotide polymorphisms (SNPs) and pseudogenes, conditions that limit INDELs' detection by Surveyor. We obtained liver-derived murine N-Muli cell clones having INDELs with efficiency close to 40%, depending on the TALEN pair and RE target site. Sequencing of the target locus and WB analysis of the isolated cell clones showed a high proportion of biallelic mutations in cells treated with the most efficient TALEN pair. Ugt glucuronidation activity was reduced basal levels in the biallelic mutant clones. These mutant liver-derived cell lines could be a very useful tool to study biochemical aspects of Ugt1 enzyme activity in a more natural context, such as substrate specificity, requirement of specific co-factors, the study of inhibitors and other pharmacological aspects, and to correlate enzyme activity to the presence of specific mutations in the gene, by adding back to the mutant cell clones specific variants of the Ugt1 gene. In addition, since genome editing has recently emerged as a potential therapeutic approach to cure genetic diseases, the definition of the most efficient TALEN pair could be an important step towards setting up a platform to perform genome editing in CNSI. [ABSTRACT FROM AUTHOR]

Published

2014

50. Allele-Specific Silencing of Mutant Huntingtin in Rodent Brain and Human Stem Cells.

Author

Drouet, Valérie, Ruiz, Marta, Zala, Diana, Feyeux, Maxime, Auregan, Gwennaëlle, Cambon, Karine, Troquier, Laetitia, Carpentier, Johann, Aubert, Sophie, Merienne, Nicolas, Bourgois-Rocha, Fany, Hassig, Raymonde, Rey, Maria, Dufour, Noëlle, Saudou, Frédéric, Perrier, Anselme L., Hantraye, Philippe, and Déglon, Nicole

Subjects

*ALLELES, *HUNTINGTIN protein, *STEM cells, *LABORATORY rodents, *HUNTINGTON disease, *POLYGLUTAMINE, *RNA interference

Abstract

Huntington's disease (HD) is an autosomal dominant neurodegenerative disorder resulting from polyglutamine expansion in the huntingtin (HTT) protein and for which there is no cure. Although suppression of both wild type and mutant HTT expression by RNA interference is a promising therapeutic strategy, a selective silencing of mutant HTT represents the safest approach preserving WT HTT expression and functions. We developed small hairpin RNAs (shRNAs) targeting single nucleotide polymorphisms (SNP) present in the HTT gene to selectively target the disease HTT isoform. Most of these shRNAs silenced, efficiently and selectively, mutant HTT in vitro. Lentiviral-mediated infection with the shRNAs led to selective degradation of mutant HTT mRNA and prevented the apparition of neuropathology in HD rat's striatum expressing mutant HTT containing the various SNPs. In transgenic BACHD mice, the mutant HTT allele was also silenced by this approach, further demonstrating the potential for allele-specific silencing. Finally, the allele-specific silencing of mutant HTT in human embryonic stem cells was accompanied by functional recovery of the vesicular transport of BDNF along microtubules. These findings provide evidence of the therapeutic potential of allele-specific RNA interference for HD. [ABSTRACT FROM AUTHOR]

Published

2014