Your search keyword '"inducible"' showing total 402 results

101. Cre-ating ways to serotonin

Author

William eWisden

Subjects

Serotonin, Tamoxifen, Tryptophan Hydroxylase, cre, 5-Hydroxytryptamine, inducible, Neurosciences. Biological psychiatry. Neuropsychiatry, RC321-571

Published

2010

102. c-Myc suppressed E-cadherin through miR-9 at the post-transcriptional level.

Author

Liu, Mei, Zhu, Hongxia, Yang, Shangbin, Wang, Zaozao, Bai, Jinfeng, and Xu, Ningzhi

Subjects

*MYC proteins, *CADHERINS, *GENETIC regulation, *MICRORNA, *GENE expression, *TRANSCRIPTION factors

Abstract

c-Myc oncoprotein is overexpressed in most human cancers and regulates different genes and pathways in different cell types. E-cadherin expression is repressed by MYC through a post-transcriptional mechanism, but the exact mechanism remains elusive. Since E-cadherin is a direct target of miR-9 and miR-9 can be activated by MYC and MYCN, this suggests that c-Myc negatively modulates E-cadherin through a microRNA pathway. We have established a c-Myc-inducible expression system in which the protein level and transcriptional activity of c-Myc is significantly upregulated upon doxycycline induction. Overexpressed c-Myc led to an EMT-like conversion in the T-REx-293 cells and resulted in a significant decrease in E-cadherin and an increase in Vimentin. Stem-loop RT-PCR showed elevated expression of miR-9 when c-Myc was induced to be overexpressed. Regarding the relationship of c-Myc, miR-9 and E-cadherin, the expression of miR-9 was curtailed by using antagomir-9 in induced overexpressing c-Myc. Restoration of E-cadherin expression became much stronger in the presence of c-Myc. Thus c-Myc represses E-cadherin at the post-transcriptional level through miR-9. [ABSTRACT FROM AUTHOR]

Published

2013

103. Inducible mouse models illuminate parameters influencing epigenetic inheritance.

Author

Wan, Mimi, Honggang Gu, Jingxue Wang, Huang, Haichang, Zhao, Jiugang, Kaundal, Ravinder K., Yu, Ming, Kushwaha, Ritu, Chaiyachati, Barbara H., Deerhake, Elizabeth, and Chi, Tian

Subjects

*ANIMAL epigenetics, *GENETIC pleiotropy, *TETRACYCLINE, *TRANSCRIPTION factors, *CHROMATIN, *LABORATORY mice

Abstract

Environmental factors can stably perturb the epigenome of exposed individuals and even that of their offspring, but the pleiotropic effects of these factors have posed a challenge for understanding the determinants of mitotic or transgenerational inheritance of the epigenetic perturbation. To tackle this problem, we manipulated the epigenetic states of various target genes using a tetracycline-dependent transcription factor. Remarkably, transient manipulation at appropriate times during embryogenesis led to aberrant epigenetic modifications in the ensuing adults regardless of the modification patterns, target gene sequences or locations, and despite lineage-specific epigenetic programming that could reverse the epigenetic perturbation, thus revealing extraordinary malleability of the fetal epigenome, which has implications for 'metastable epialleles'. However, strong transgenerational inheritance of these perturbations was observed only at transgenes integrated at the Col1a1 locus, where both activating and repressive chromatin modifications were heritable for multiple generations; such a locus is unprecedented. Thus, in our inducible animal models, mitotic inheritance of epigenetic perturbation seems critically dependent on the timing of the perturbation, whereas transgenerational inheritance additionally depends on the location of the perturbation. In contrast, other parameters examined, particularly the chromatin modification pattern and DNA sequence, appear irrelevant. [ABSTRACT FROM AUTHOR]

Published

2013

104. Inducible CRISPR/Cas9 Allows for Multiplexed and Rapidly Segregated Single-Target Genome Editing in Synechocystis Sp. PCC 6803.

Author

Cengic I, Cañadas IC, Minton NP, and Hudson EP

Subjects

CRISPR-Cas Systems genetics, DNA-Binding Proteins genetics, Endoribonucleases genetics, Escherichia coli genetics, Gene Editing, Nickel, Theophylline, Escherichia coli Proteins genetics, Riboswitch, Synechocystis genetics

Abstract

Establishing various synthetic biology tools is crucial for the development of cyanobacteria for biotechnology use, especially tools that allow for precise and markerless genome editing in a time-efficient manner. Here, we describe a riboswitch-inducible CRISPR/Cas9 system, contained on a single replicative vector, for the model cyanobacterium Synechocystis sp. PCC 6803. A theophylline-responsive riboswitch allowed tight control of Cas9 expression, which enabled reliable transformation of the CRISPR/Cas9 vector into Synechocystis . Induction of the CRISPR/Cas9 mediated various types of genomic edits, specifically deletions and insertions of varying size. The editing efficiency varied depending on the target and intended edit; smaller edits performed better, reaching, e.g., 100% for insertion of a FLAG-tag onto rbcL . Importantly, the single-vector CRISPR/Cas9 system mediated multiplexed editing of up to three targets in parallel in Synechocystis . All single-target and several double-target mutants were also fully segregated after the first round of induction. Lastly, a vector curing system based on the nickel-inducible expression of the toxic mazF (from Escherichia coli ) was added to the CRISPR/Cas9 vector. This inducible system allowed for curing of the vector in 25-75% of screened colonies, enabling edited mutants to become markerless.

Published

2022

105. Direct conversion of human fibroblast to hepatocytes using a single inducible polycistronic vector

Author

Ballester, Maria, Bolonio, Miguel, Santamaria, Ramon, Castell, José V., Ribes-Koninckx, Carmen, and Bort, Roque

Published

2019

106. The androgen receptor is required for maintenance of bone mass in adult male mice

Author

Wu, J. (Jianyao), Henning, P. (Petra), Sjögren, K. (Klara), Koskela, A. (Antti), Tuukkanen, J. (Juha), Movérare-Skrtic, S. (Sofia), Ohlsson, C. (Claes), Wu, J. (Jianyao), Henning, P. (Petra), Sjögren, K. (Klara), Koskela, A. (Antti), Tuukkanen, J. (Juha), Movérare-Skrtic, S. (Sofia), and Ohlsson, C. (Claes)

Abstract

Previous studies evaluating the role of the androgen receptor (AR) for bone mass have used mouse models with global or tissue-specific lifelong inactivation of the AR. However, these mouse models have the AR inactivated already early in life and the relative roles of the AR during development, sexual maturation and in adult mice cannot be evaluated separately. The aim of the present study was to determine the specific roles of the AR in bone during sexual maturation and in adult mice. The AR was conditionally ablated at four (pre-pubertal) or ten (post-pubertal) weeks of age in male mice using tamoxifen-inducible Cre-mediated recombination. Both the pre-pubertal and the post-pubertal AR inactivation were efficient demonstrated by substantially lower AR mRNA levels in seminal vesicle, bone and white adipose tissue as well as markedly reduced weights of reproductive tissues when comparing inducible ARKO mice and control mice at 14 weeks of age. Total body BMD, as analyzed by DXA, as well as tibia diaphyseal cortical bone thickness and proximal metaphyseal trabecular bone volume fraction, as analyzed by μCT, were significantly reduced by both pre-pubertal and post-pubertal AR inactivation. These bone effects were associated with an increased bone turnover, indicating a high bone turnover osteoporosis. Pre-pubertal but not post-pubertal AR inactivation resulted in substantially increased fat mass. In conclusion, the AR is required for maintenance of both trabecular and cortical bone in adult male mice while AR expression during puberty is crucial for normal fat mass homeostasis in adult male mice.

Published

2019

107. Construction of over-expression shuttle vectors in Streptomyces.

Author

Sun, Ning, Wang, Zhi-Bin, Wu, He-Ping, Mao, Xu-Ming, and Li, Yong-Quan

Abstract

Two high-copy number vectors, pL97 and pL98, that contain the strong constitutive ermEp* from Saccharopolyspora erythraea and the ssrA promoter ( ssrAp) from Streptomyces coelicolor, respectively, and an inducible high-copy vector, pL99, with the PnitA-NitR system from Rhodococcus rhodochrous, were constructed based on the pIJ101 replicon. These vectors have pUC18 and pIJ101 replication origins for high-copy plasmid number in Escherichia coli and Streptomyces, respectively, and the oriT (RK2) allows the efficient and convenient plasmid transfer from E. coli to Streptomyces. The transformants can be easily selected with apramycin. There is also a multiple cloning site (MCS) between promoter and terminator convenient for heterologous gene cloning. The enhanced green fluorescent protein (EGFP) gene and redD, a pathway-specific regulatory gene for the production of undecylprodigiosin in S. coelicolor, were inserted into these plasmids and could be over-expressed in S. coelicolor. Western blotting revealed that the expression of EGFP was dramatically increased compared to the cell with a single copy of EGFP. Furthermore, the production of undecylprodigiosin was also greatly enhanced in the cells constitutively over-expressing redD. Hence, the high-copy plasmids could be readily used to express foreign proteins and for production of secondary metabolites, especially the antibiotics, potentially for industrial applications. [ABSTRACT FROM AUTHOR]

Published

2012

108. Use of inducible Atg5 deletion and expression cell lines in study of the pro-survival function of autophagy under starvation

Author

Chen, Bo, Sun, Xiangjie, Zhang, Yin, Zhu, Xin-Qiang, and Shen, Han-Ming

Subjects

*CELL lines, *GENE expression, *AUTOPHAGY, *FIBROBLASTS, *CELL death, *CHLOROQUINE, *LABORATORY mice

Abstract

Abstract: At present the role of autophagy in cell death and cell survival remains controversial, partly owning to the contradictory results from the immortalized mouse embryonic fibroblasts (MEFs) with knockout of different autophagy-related genes (Atg). Here we aimed to reexamine the role of autophagy in cell death under starvation and other stress conditions. First, different clones of Atg5 knockout MEFs had different susceptibility to stress-mediated cell death, indicating that it is the clonal variation, rather than the deficiency of Atg5 or autophagy per se that determines the susceptibility. Next, we tested two cell lines with inducible Atg5 deletion or expression and demonstrated that cells without Atg5 expression were more sensitive to starvation-induced apoptosis. Finally, we found that chloroquine was only effective in sensitizing starvation-induced cell death in Atg5-expressing cells, but not in Atg5-deficient cells. Such observations thus provide unequivocal evidence supporting the pro-survival function of autophagy under starvation. Moreover, our data demonstrate the usefulness of cells with inducible deletion or expression of Atg in the study of autophagy in cell death and cell survival. [Copyright &y& Elsevier]

Published

2012

109. A single plasmid transfection that offers a significant advantage associated with puromycin selection, fluorescence-assisted cell sorting, and doxycycline-inducible protein expression in mammalian cells.

Author

Iwaki, Takayuki and Umemura, Kazuo

Abstract

lthough there are several inducible expression systems for mammalian cells, the most reliable one is the tetracycline-regulated expression system. This system is well-established and widely used by many researchers. Although Clontech provides several types of cells that stably express reverse tetracycline transactivator (rtTA), the cells that are not provided can be generated with pTet-On-Advanced by first integrating this plasmid into the require type of cell and then introducing the genes of interest. These processes are experimental bottlenecks. To improve this situation, we synthesized an all-in-one vector, termed pMAK17, which enables constitutive expression of puromycin N-acetyltransferase, modified Discosoma red fluorescent protein, and rtTA, as well as P-driven enhanced green fluorescent protein (EGFP). The pMAK17-transfected cells could be successfully induced to express EGFP, were selectable by fluorescence-activated cell sorting, and displayed puromycin resistance. [ABSTRACT FROM AUTHOR]

Published

2011

110. Gene Expression Profile Associated with Oncogenic Ras-induced Senescence, Cell Death, and Transforming Properties in Human Cells.

Author

Moumtzi, Sophy S., Roberts, Michael L., Joyce, Tobias, Evangelidou, Maria, Probert, Lesley, Frillingos, Stathis, Fotsis, Theodore, and Pintzas, Alexander

Subjects

*GENE expression, *GENETIC regulation, *CELL death, *CELL cycle, *INTEGRINS, *APOPTOSIS

Abstract

We developed inducible and constitutive expression systems of Ha-RasV12 in HEK 293 cells to examine early oncogenic RasV12 signaling. Inducible expression of oncogenic Ras-triggered growth arrest, early senescence, and later apoptosis. Gene expression profile analysis revealed early Ras proliferation and cell cycle genes like c-fos, cyclin E, cdk2, cell–cell contact, and signaling like integrin a6, MEK5, and free radical signaling genes, like proline oxidase. Therefore, Ras-mediated signaling is a fine regulated process both positively and negatively influencing cell cycle, senescence, and apoptosis pathways. Novel early RAS-target genes could be potentially exploited in cancer diagnostics and therapeutics. [ABSTRACT FROM AUTHOR]

Published

2010

111. Promoter diversity in multigene transformation.

Author

Peremarti, Ariadna, Twyman, Richard M., Gómez-Galera, Sonia, Naqvi, Shaista, Farré, Gemma, Sabalza, Maite, Miralpeix, Bruna, Dashevskaya, Svetlana, Yuan, Dawei, Ramessar, Koreen, Christou, Paul, Zhu, Changfu, Bassie, Ludovic, and Capell, Teresa

Abstract

Multigene transformation (MGT) is becoming routine in plant biotechnology as researchers seek to generate more complex and ambitious phenotypes in transgenic plants. Every nuclear transgene requires its own promoter, so when coordinated expression is required, the introduction of multiple genes leads inevitably to two opposing strategies: different promoters may be used for each transgene, or the same promoter may be used over and over again. In the former case, there may be a shortage of different promoters with matching activities, but repetitious promoter use may in some cases have a negative impact on transgene stability and expression. Using illustrative case studies, we discuss promoter deployment strategies in transgenic plants that increase the likelihood of successful and stable multiple transgene expression. [ABSTRACT FROM AUTHOR]

Published

2010

112. Temporal requirement of RPE-derived VEGF in the development of choroidal vasculature.

Author

Yun-Zheng Le, Yanyan Bai, Meili Zhu, and Lixin Zheng

Subjects

*CYTOKINES, *GROWTH factors, *IMMUNOBLOTTING, *IMMUNOHISTOCHEMISTRY, *ELECTRODIAGNOSIS

Abstract

J. Neurochem. (2010) 112, 1584–1592. Vascular endothelial growth factor (VEGF-A or VEGF) is a potent growth factor for the development of retinal and choroidal vasculatures. To define the temporal requirement of the retinal pigmented epithelium (RPE)-derived VEGF in choroidal vascular development, we generated conditional VEGF knockout mice using an inducible Cre/ lox system. The loss of the RPE-derived VEGF was confirmed with immunoblotting and immunohistochemistry. Retinal function and structure were assessed with electroretinography and histology, respectively. Choroidal vascular density was analyzed with computer-assisted semi-quantitative assay using fluorescently labeled choroidal flat-mounts. Induction of RPE-specific VEGF disruption at embryonic day 10 (E10) or E13 for 2 days caused regulatable decreases in choroidal vascular density, photoreceptor function, and photoreceptor outer nuclear layer thickness. The loss of the RPE-produced VEGF after E15 did not cause detectable defects in choroidal vasculatures and photoreceptor function and morphology. These results suggest that the RPE-derived VEGF plays a critical role in choroidal vascular development during organogenesis before E15. [ABSTRACT FROM AUTHOR]

Published

2010

113. Purification and Characterization of a Novel Heparin Degrading Enzyme from Aspergillus flavus (MTCC-8654).

Author

Banga, Jaspreet and Tripathi, C. K. M.

Abstract

A heparinase-producing fungus was isolated, and the strain was taxonomically characterized as Aspergillus flavus by morphophysiological and 26S rRNA gene homology studies. The culture produced intracellular heparinase enzyme, which was purified 40.5-fold by DEAE-Sephadex A-50, CM-Sephadex C-50, and Sephadex G-100 column chromatography. Specific activity of the purified enzyme was found to be 44.6 IU/µg protein and the molecular weight of native as well as reduced heparinase was 24 kDa, showing a monomeric unit structure. Peptide mass spectrum showed poor homogeneity with the database in the peptide bank. The enzyme activity was maximum at 30 °C in the presence of 300 mM NaCl at pH 7.0. In the presence of Co2+, Mn2+ ions, and reducing agents (β- mercaptoethanol, dithiothreitol), enzyme activity was enhanced and inhibited by iodoacetic acid. These observations suggested that free sulfohydryl groups of cysteine residues were necessary for catalytic activity of the enzyme. The enzyme was also inhibited by histidine modifier, DEPC, which suggests that along with cysteine, histidine may be present at its active site. The enzyme showed a high affinity for heparin as a substrate with Km and Vmax as 2.2x10-5 M and 30.8 mM min-1, respectively. The affinity of the enzyme for different glycosaminoglycans studied varied, with high substrate specificity toward heparin and heparin-derived polysaccharides. Depolymerization of heparin and fractionation of the oligosaccharides yielded heparin disaccharides as main product. [ABSTRACT FROM AUTHOR]

Published

2010

114. Nucleocytoplasmic plant lectins

Author

Lannoo, Nausicaä and Van Damme, Els J.M.

Subjects

*PLANT lectins, *CARBOHYDRATES, *CARRIER proteins, *AGGLUTININS, *EFFECT of stress on plants, *CYTOPLASM, *CELL nuclei, *PLANT cells & tissues

Abstract

Abstract: During the last decade it was unambiguously shown that plants synthesize minute amounts of carbohydrate-binding proteins upon exposure to stress situations like drought, high salt, hormone treatment, pathogen attack or insect herbivory. In contrast to the ‘classical’ plant lectins, which are typically found in storage vacuoles or in the extracellular compartment this new class of lectins is located in the cytoplasm and the nucleus. Based on these observations the concept was developed that lectin-mediated protein–carbohydrate interactions in the cytoplasm and the nucleus play an important role in the stress physiology of the plant cell. Hitherto, six families of nucleocytoplasmic lectins have been identified. This review gives an overview of our current knowledge on the occurrence of nucleocytoplasmic plant lectins. The carbohydrate-binding properties of these lectins and potential ligands in the nucleocytoplasmic compartment are discussed in view of the physiological role of the lectins in the plant cell. [Copyright &y& Elsevier]

Published

2010

115. Prevalence of erm methylase genes in clinical isolates of non-pigmented, rapidly growing mycobacteria.

Author

Esteban, J., Martín-de-Hijas, N. Z., García-Almeida, D., Bodas-Sánchez, Á., Gadea, I., and Fernández-Roblas, R.

Subjects

*MYCOBACTERIUM, *ACTINOMYCETALES, *HEREDITY, *THERAPEUTICS, *INFECTION

Abstract

The aim of this study was to determine the frequency of erm genes coding for macrolide resistance among clinical isolates of non-pigmented rapidly growing mycobacteria (NPRGM) and to evaluate their importance in phenotypic resistance. Broth microdilution susceptibility testing was performed for all NPRGM tested. A PCR assay with consensus primers was used to evaluate the presence of erm genes among the 167 clinical isolates studied, which belonged to nine species of NPRGM; erm genes were detected in all nine species and 109 strains were erm-positive. The highest percentage of erm-positive isolates was found among Mycobacterium mageritense (100%) and the lowest among Mycobacterium mucogenicum (14%). The MICs of macrolides were found to be lower for erm-negative isolates (MIC90: 2 mg/L) than for erm-positive isolates (MIC90: 16 mg/L), although in some cases high MICs were found for erm-negative isolates. The finding that erm methylases are present in the majority of the species of NPRGM analysed in this study is not in agreement with conventional susceptibility studies. It therefore appears necessary to use a combination therapy to treat infections caused by NPRGM. [ABSTRACT FROM AUTHOR]

Published

2009

116. Cyclooxygenase in normal human tissues – is COX-1 really a constitutive isoform, and COX-2 an inducible isoform?

Author

Zidar, Nina, Odar, Katarina, Glavač, Damjan, Jerše, Maja, Zupanc, Tomaz, and Štajer, Dusan

Subjects

CYCLOOXYGENASE 2, SMOOTH muscle, IMMUNOHISTOCHEMISTRY, CYCLOOXYGENASES, BLOOD platelets

Abstract

Cyclooxygenase (COX) is a key enzyme in prostanoid synthesis. It exists in two isoforms, COX-1 and COX-2. COX-1 is referred to as a ‘constitutive isoform’, and is considered to be expressed in most tissues under basal conditions. In contrast, COX-2 is referred to as an ‘inducible isoform’, which is believed to be undetectable in most normal tissues, but can be up-regulated during various conditions, many of them pathological. Even though the role of COX in homeostasis and disease in now well appreciated, controversial information is available concerning the distribution of COX isoforms in normal human tissues. There is mounting evidence that it is much more complex than generally believed. Our aim was therefore to analyse the expression and distribution of COX isoforms in normal human tissues, using immunohistochemistry, Western blotting and real-time RT-PCR. Autopsy samples from 20 healthy trauma victims and samples from 48 biopsy surgical specimens were included. COX-1 was found in blood vessels, interstitial cells, smooth muscle cells, platelets and mesothelial cells. In contrast, COX-2 was found predominantly in the parenchymal cells of many tissues, with few exceptions, for example the heart. Our results confirm the hypothesis that the distribution of COX isoforms in healthy tissues is much more complex than generally believed. This and previous studies indicate that both isoforms, not only COX-1, are present in many normal human tissues, and that both isoforms, not only COX-2, are up-regulated in various pathological conditions. We may have to revise the concept of ‘constitutive’ and ‘inducible’ COX isoforms. [ABSTRACT FROM AUTHOR]

Published

2009

117. Isolation of a Latimeria menadoensis heat shock protein 70 ( Lmhsp70) that has all the features of an inducible gene and encodes a functional molecular chaperone.

Author

Modisakeng, Keoagile W., Jiwaji, Meesbah, Pesce, Eva-Rachele, Robert, Jacques, Amemiya, Chris T., Dorrington, Rosemary A., and Blatch, Gregory L.

Subjects

*MOLECULAR chaperones, *PROTEINS, *LATIMERIA menadoensis, *HEAT shock proteins, *ADENOSINE triphosphatase

Abstract

Molecular chaperones facilitate the correct folding of other proteins, and heat shock proteins form one of the major classes of molecular chaperones. Heat shock protein 70 (Hsp70) has been extensively studied, and shown to be critically important for cellular protein homeostasis in almost all prokaryotic and eukaryotic systems studied to date. Since there have been very limited studies conducted on coelacanth chaperones, the main objective of this study was to genetically and biochemically characterize a coelacanth Hsp70. We have successfully isolated an Indonesian coelacanth ( L. menadoensis) hsp70 gene, Lmhsp70, and found that it contained an intronless coding region and a potential upstream regulatory region. Lmhsp70 encoded a typical Hsp70 based on conserved structural and functional features, and the predicted upstream regulatory region was found to contain six potential promoter elements, and three potential heat shock elements (HSEs). The intronless nature of the coding region and the presence of HSEs suggested that Lmhsp70 was stress-inducible. Phylogenetic analyses provided further evidence that Lmhsp70 was probably inducible, and that it branched as a clade intermediate between bony fish and tetrapods. Recombinant LmHsp70 was successfully overproduced, purified and found to be functional using ATPase activity assays. Taken together, these data provide evidence for the first time that the coelacanth encodes a functional molecular chaperone system. [ABSTRACT FROM AUTHOR]

Published

2009

118. Treatment of diabetes by transplantation of drug-inducible insulin-producing gut cells.

Author

Unniappan, Suraj, Wideman, Rhonda D., Donald, Christine, Gunn, Virginia, Wall, Jennifer L., Zhang, Qiu-Xia, Webber, Travis D., Cheung, Anthony T., and Kieffer, Timothy J.

Subjects

*TREATMENT of diabetes, *INSULIN, *BLOOD sugar, *CELL lines, *MIFEPRISTONE, *MESSENGER RNA, *C-peptide, *CELL transplantation

Abstract

Most patients with type 1 diabetes rely on multiple daily insulin injections to maintain blood glucose control. However, insulin injections carry the risk of inducing hypoglycemia and do not eliminate diabetic complications. We sought to develop and evaluate a regulatable cell-based system for delivery of insulin to treat diabetes. We generated two intestinal cell lines in which human insulin expression is controlled by mifepristone. Insulin mRNA expression was dependent on the mifepristone dose and incubation time and cells displayed insulin and C-peptide immunoreactivity and glucose-induced insulin release following mifepristone treatment. Cell transplantation followed by mifepristone administration reversed streptozotocin (STZ)-induced diabetes in mice, and this effect was dependent on the mifepristone dose delivered. These data support the notion that engineering regulatable insulin expression within a cell already equipped for regulated secretion may be efficacious for the treatment of insulin-dependent diabetes. [ABSTRACT FROM AUTHOR]

Published

2009

119. Endothelin receptor blockade does not affect blood pressure or angiotensin II levels in CYP1A1-Ren-2 transgenic rats with acutely induced hypertension

Author

Vaňourková, Zdeňka, Kramer, Herbert J., Erbanová, Michaela, Bäcker, Angela, Červenka, Luděk, Husková, Zuzana, Chábová, Věra Čertíková, Tesař, Vladimír, Dvořák, Pavel, Malý, Jan, and Vaněčková, Ivana

Subjects

*ENDOTHELINS, *BLOOD pressure, *LABORATORY rats, *ANGIOTENSIN II, *HYPERTENSION, *BODY weight, *TRANSGENIC mice

Abstract

Abstract: We found previously that selective blockade of endothelin ETA receptors is superior to nonselective ETA/ETB in attenuating hypertension and survival rate in Ren-2 transgenic rats (TGR). In the present pilot study, we were interested in whether similar effects will be found in TGR with inducible malignant hypertension (iTGR; official strain name Cyp1A1-Ren-2rats), which were derived from the original Ren-2 transgenic rat strain. Studies were performed in three-month old male iTGR. Treatment with either bosentan, a non-selective ETA/ETB, or with atrasentan, a selective ETA receptor blocker, was started on day 2 of the experiment. Feeding with indole-3-carbinole (I3C; 0.3% in rat chow), a natural xenobiotic which activates the Cyp1a1 promoter of the mouse Ren-2 gene, began on day 3 and lasted for 4 days until day 6. Systolic BP, body weight, plasma ANG II and tissue ANG II and ET-1 concentrations were determined daily. Severe hypertension developed as early as 1 day after beginning of I3C feeding which was accompanied by a significant reduction in body weight and by increases in plasma and tissue ANG II and left ventricle ET-1 concentrations. Atrasentan or bosentan had no effects on the rise in BP or plasma and tissue ANG II concentrations but prevented the rise in heart ventricle ET-1 concentration. Our data show that blockade of the ET system does not prevent or attenuate the rapid development of severe hypertension in iTGR; a long-term protective effect of ET blockade on cardiac (and renal) damage, however, cannot be excluded and awaits further investigations. [Copyright &y& Elsevier]

Published

2009

120. A calpain unique to alveolates is essential in Plasmodium falciparum and its knockdown reveals an involvement in pre-S-phase development.

Author

Russo, Ilaria, Oksman, Anna, Vaupel, Barbara, and Goldberg, Daniel E.

Subjects

*CALPAIN, *PLASMODIUM falciparum, *TARGETED drug delivery, *PROTEOLYTIC enzyme genes, *CELL cycle regulation, *CYSTEINE proteinases

Abstract

Plasmodium falciparum encodes a single calpain that has a distinct domain composition restricted to alveolates. To evaluate the potential of this protein as a drug target, we assessed its essentiality. Both gene disruption by double cross-over and gene truncation by single cross-over recombination failed. We were also. unable to achieve allelic replacement by using a missense mutation at the catalytic cysteine codon, although we could obtain synonymous allelic replacement parasites. These results suggested that the calpain gene and its proteolytic activity are important for optimal parasite growth. To gain further insight into its biological role, we used the FKBP degradation domain system to generate a fusion protein whose stability in transfected parasites could be modulated by a small FKBP ligand, Shieldi (ShId1). We made a calpain-GFP-FKBP fusion through single cross-over integration at the endogenous calpain locus. Calpain levels were knocked down and parasite growth was greatly impaired in the absence of ShId1. Parasites were delayed in their ability to transition out of the ring stage and in their ability to progress to the S phase. Calpain is required for cell cycle progression in Plasmodium parasites and appears to be an attractive drug target. We have shown that regulated knockdowns are possible in P. fakiparum and can be useful for evaluating essentiality and function. [ABSTRACT FROM AUTHOR]

Published

2009

121. Macrolide–lincosamide–streptogramin B resistance phenotypes in clinical staphylococcal isolates

Author

Cetin, Emel Sesli, Gunes, Hayati, Kaya, Selcuk, Aridogan, Buket Cicioglu, and Demirci, Mustafa

Subjects

*STAPHYLOCOCCAL diseases, *ANTI-infective agents, *ANTIBIOTICS, *PHENOTYPES

Abstract

Abstract: The prevalence of macrolide–lincosamide–streptogramin B (MLSB) resistance as well as the MLSB resistance phenotypes were investigated by the double-disk diffusion test among 532 clinical staphylococci isolates in a Turkish university hospital. The activity of other antimicrobials, including trimethoprim/sulfamethoxazole, telithromycin, quinupristin/dalfopristin, linezolid, gentamicin, chloramphenicol, ciprofloxacin and vancomycin, was also evaluated. Of 532 isolates, 38.5% were resistant to MLSB antibiotics; 63.9% of the resistant isolates exhibited a constitutive phenotype (cMLSB) whereas 36.1% expressed an inducible resistance phenotype (iMLSB). MLSB resistance was more prevalent among coagulase-negative staphylococci (CoNS) strains. Oxacillin-resistant strains exhibited significantly higher MLSB resistance rates compared with oxacillin-susceptible strains (P <0.0001). The most frequently detected resistance phenotype among the total staphylococcal isolates was the constitutive type and this phenotype was more frequently encountered among oxacillin-resistant strains. With the exception of the fully active agents such as vancomycin, linezolid and quinupristin/dalfopristin, the most effective antibiotics were telithromycin and chloramphenicol among all isolates. Susceptibility rates to other antibiotics tested were higher among isolates without MLSB resistance than isolates with MLSB resistance. The detection of a considerable rate (43.5%) of iMLSB resistance among erythromycin-resistant/clindamycin-susceptible strains suggests that the true percentage of clindamycin resistance may be underestimated if testing for inducible resistance is not performed. [Copyright &y& Elsevier]

Published

2008

122. Oncogene cooperation in tumor maintenance and tumor recurrence in mouse mammary tumors induced by Myc and mutant Kras.

Author

Podsypanina, Katrina, Politi, Katerina, Beverly, Levi J., and Varmus, Harold E.

Subjects

*IMMUNOGENETICS, *MYC oncogenes, *GENETIC mutation, *MAMMARY gland cancer, *GENETICS of breast cancer, *GENE expression

Abstract

Most, if not all, cancers are composed of cells in which more than one gene has a cancer-promoting mutation. Although recent evidence has shown the benefits of therapies targeting a single mutant protein, little attention has been given to situations in which experimental tumors are induced by multiple cooperating oncogenes. Using combinations of doxycycline-inducible and constitutive Myc and mutant Kras transgenes expressed in mouse mammary glands, we show that tumors induced by the cooperative actions of two oncogenes remain dependent on the activity of a single oncogene. Deinduction of either oncogene individually, or both oncogenes simultaneously, led to partial or complete tumor regression. Prolonged remission followed deinduction of KrasG12D in the context of continued Myc expression, deinduction of a MYC transgene with continued expression of mutant Kras produced modest effects on life extension, whereas simultaneous deinduction of both MYC and KrasG12D transgenes further improved survival. Disease relapse after deinduction of both oncogenes was associated with reactivation of both oncogenic transgenes in all recurrent tumors, often in conjunction with secondary somatic mutations in the tetracycline transactivator transgene, MMTV- rtTA, rendering gene expression doxycycline-independent. These results demonstrate that tumor viability is maintained by each gene in a combination of oncogenes and that targeted approaches will also benefit from combination therapies. [ABSTRACT FROM AUTHOR]

Published

2008

123. Inducible antiviral activity and rapid production of the Ribosome-Inactivating Protein I from Phytolacca heterotepala in tobacco

Author

Corrado, Giandomenico, Scarpetta, Mariarosaria, Alioto, Daniela, Di Maro, Antimo, Polito, Letizia, Parente, Augusto, and Rao, Rosa

Subjects

*PLANT resistance to viruses, *TOBACCO, *PLANT hormones, *GENE expression

Abstract

Abstract: We studied the in vitro and in planta antiviral activity of the PhRIP I, a type 1 Ribosome-Inactivating Protein originally purified from leaves of the Phytolacca heterotepala. This protein inhibited protein translation in a cell-free assay and limited the local lesion formation from PVX infection on tobacco leaves. We used a transient expression system based on leaf infiltration with recombinant Agrobacteria to show that tobacco can produce a correctly processed PhRIP I enzyme that retains its antiviral activity. Hence, it is possible to rapidly yield in plants a type 1 RIP by means of this transient expression system. To analyse the possible increase of virus resistance in plants, Nicotiana tabacum lines that were transformed with the PhRIP I coding sequence under the control of the wound-inducible PGIP promoter were challenged by PVX. A significantly lower number of viral lesions compared to untransformed plants was observed only after the induction of the transgene, indicating that the controlled gene expression of an antiviral protein can increase virus resistance. [Copyright &y& Elsevier]

Published

2008

124. Sulfur mustard downregulates iNOS expression to inhibit wound healing in a human keratinocyte model

Author

Ishida, Hiroshi, Ray, Radharaman, and Ray, Prabhati

Subjects

*KERATINOCYTES, *CELLS, *NITRIC oxide, *NITROGEN compounds

Abstract

Summary: Background: Increased nitric oxide (NO) synthesized by inducible NO synthase (iNOS) is involved in inflammatory and pathological conditions. iNOS also regulates several biomarkers that accelerate normal wound healing. Effects of exposure to sulfur mustard (SM) on the skin include formation of blisters and slow-healing injuries. Promoting re-epithelialization is a challenging issue in the treatment of the delayed healing of SM-induced skin injuries. Objectives: To clarify the role(s) of iNOS in wound healing and the effect of SM on iNOS expression in an in vitro wound assay to eventually develop therapies for SM skin injuries. Methods: A wound was created by scratching normal human epidermal keratinocytes grown in vitro. iNOS expression was monitored by Western blotting, fluorescence microscopy, and real-time RT-PCR. Wound healing was analyzed using digitalized image analysis software. Results: The level of iNOS peaked 24–48h after wounding. SM exposure strongly reduced iNOS protein and mRNA levels. Fluorescence microscopy revealed that induction of iNOS expression by wounding and inhibition of iNOS expression by SM occurred not only in the cells at the wound edge but also in cells in the surrounding area, suggesting that wounding may induce and SM may inhibit release of cytokines that stimulate iNOS expression. iNOS-specific small interfering RNAs caused a marked decrease of iNOS expression irrespective of wounding. Gene silencing also completely inhibited wound healing. Conclusion: These results suggest that preventing SM-induced inhibition of iNOS may be a prospective strategy to promote wound healing in SM-exposed skin. [Copyright &y& Elsevier]

Published

2008

125. Specific developmental disruption of disrupted-in-schizophrenia-i function results in schizophrenia-related phenotypes in mice.

Author

Weidong Li, Yu Zhou, Jentsch, J. David, Brown, Robert A. M., Xiaoli Tian, Ehninger, Dan, Hennah, William, Peltonen, Leena, Lonnqvist, Jouko, Huttunen, Matti O., Kaprio, Jaakko, Trachtenberg, Joshua T., Silva, Alcino J., and Cannon, Tyrone D.

Subjects

*TRANSGENIC mice, *MENTAL depression, *SHORT-term memory, *SOCIABILITY, *SCHIZOPHRENIA

Abstract

Disrupted-in-schizophrenia 1 (DISC1) was initially discovered through a balanced translocation (1;11)(q42.1;q14.3) that results in loss of the C terminus of the DISC1 protein, a region that is thought to play an important role in brain development. Here, we use an inducible and reversible transgenic system to demonstrate that early postnatal, but not adult induction, of a C-terminal portion of DISC1 in mice results in a cluster of schizophrenia-related phenotypes, including reduced hippocampal dendritic complexity, depressive-like traits, abnormal spatial working memory, and reduced sociability. Accordingly, we report that individuals in a discordant twin sample with a DISC1 haplotype, associating with schizophrenia as well as working memory impairments and reduced gray matter density, were more likely to show deficits in sociability than those without the haplotype. Our findings demonstrate that alterations in DISC1 function during brain development contribute to schizophrenia pathogenesis. [ABSTRACT FROM AUTHOR]

Published

2007

126. Coculture-inducible bacteriocin activity of Lactobacillus plantarum strain J23 isolated from grape must

Author

Rojo-Bezares, Beatriz, Sáenz, Yolanda, Navarro, Laura, Zarazaga, Myriam, Ruiz-Larrea, Fernanda, and Torres, Carmen

Subjects

*LACTOBACILLUS, *PROTEOLYTIC enzymes, *DIGESTIVE enzymes, *PROKARYOTES

Abstract

Abstract: Detection and characterization of bacteriocin production by Lactobacillus plantarum strain J23, recovered from a grape must sample in Spain, have been carried out. Bacteriocin activity was degraded by proteolytic enzymes (trypsin, alfa-chymotrypsin, papaine, protease, proteinase K and acid proteases), and it was stable at high temperatures (121°C, 20min), in a wide range of pH (1–12), and after treatment with organic solvents. L. plantarum J23 showed antimicrobial activity against Oenococcus oeni, and a range of Lactobacillus and Pediococcus species. Bacteriocin production was detected in liquid media only when J23 was cocultivated with some inducing bacteria, and induction took place when intact cells or 55°C heated cells of the inducer were cocultivated with J23, but not with their autoclaved cells. Bacteriocin activity of J23 was not induced by high initial J23 inocula, and it was detected in cocultures during the exponential phase. The presence of ethanol or acidic pH in the media reduced bacteriocin production in the cocultures of J23 with the inducing bacteria. The presence of plantaricin-related plnEF and plnJ genes was detected by PCR and sequencing. Nevertheless, negative results were obtained for plnA, plnK, plNC8, plS and plW genes. [Copyright &y& Elsevier]

Published

2007

127. Measurement of natural (CD+CDhigh) and inducible (CD4+IL-10+) regulatory T cells in patients with systemic lupus erythematosus.

Author

Barath, S., Aleksza, M., Tarr, T., Sipka, S., Szegedi, G., and Kiss, E.

Subjects

*SYSTEMIC lupus erythematosus, *T cells, *CELL populations, *PATIENTS, *IMMUNOMODULATORS, *FLOW cytometry

Abstract

Abnormalities of regulatory T cells may play an important role in the loss of self-tolerance, which is a major characteristic of lupus. The objective of this study was to determine the ratio and the number of natural CD4+CD25highFoxp3+ and inducible CD4+IL-10+ regulatory T cells in lupus patients and to search correlation with disease activity. Seventy-two Hungarian lupus patients were enrolled in the study. Fourty-one age- and sex matched healthy donors served as controls. Flow cytometry was used for the quantification of CD4+CD25highFoxp3+ (nTreg) and CD4+IL-10+ (iTreg) cells. The ratio (3.06 ± 1.45%) and the number (0.019 ± 0.012 × 109⁄L) of nTreg cells decreased in lupus significantly (P < 0.001 in both) as compared to normal controls (4.26 ± 1.01% and 0.039 ± 0.017 × 109⁄L). The ratio of iTreg cells were significantly higher in patients than in controls (20.92 ± 14.02% versus 15.49 ± 11.65%, P < 0.03), but the number of these cell type did not differ in significant manner (0.314 ± 0.236 × 109⁄L versus 0.259 ± 0.183 × 109⁄L). The 19 active patients were characterised by significantly higher disease activity index (SLEDAI 8.63 ± 2.95 versus 1.74 ± 1.68, P < 0.001) and anti-DNA concentration (117.85 ± 145.89 versus 37.36 ± 68.85 IU/mL, P = 0.001) as compered to the 52 inactive patients. Furthermore, active patients required higher dose of methylprednisolon than inactive ones (14.8 ± 10.6 versus 4.8 ± 3.4 mg/day, P = 0.001). However, we did not find statistical significant difference in the number and ratio of the examined cell populations regarding to disease activity. Altered ratio and number of both natural and inducible regulatory T cells may play a role in the pathogenesis of lupus. There are small but appreciable difference in the number of regulatory T cells between inactive patients and healthy controls. It suggests that immunoregulatory deficiencies are present in the inactive stage of the disease also. [ABSTRACT FROM AUTHOR]

Published

2007

128. Selective iNOS inhibition enhances spontaneous gallbladder motility in the Australian possum.

Author

Woods, C. M., Sandstrom, P., Bond, M., Michael, M., Svanvik, J., Toouli, J., and Saccone, G. T. P.

Subjects

*NITRIC oxide, *CHOLECYSTITIS, *PHALANGERIDAE, *POLYMERASE chain reaction, *GENE expression

Abstract

Gallbladder inflammation is a common and painful disease. Inducible nitric oxide synthase (iNOS) plays a major role in inflammatory diseases, and iNOS inhibitors are being developed as therapeutic agents. Reports are inconsistent regarding iNOS expression in normal gallbladder. The aim of this study was to determine the effect of iNOS inhibition on spontaneous gallbladder motility. mRNA extracted from normal possum gallbladders was analysed by PCR. Gallbladder contractility was evaluated using a highly selective iNOS inhibitor AR-C102222AA (AR-C) in in vitro muscle strips (0.1–10 000 μm) and in vivo (0.1–30 μmol kg−1) experiments. Gene expression analysis revealed the presence of iNOS mRNA in normal gallbladder ( n = 3). In vitro, AR-C (0.1–1000 μmol L−1) produced a concentration-dependent increase in spontaneous gallbladder contractile activity and basal tension ( P < 0.05; n = 6). The maximum effect was a 1.8-fold increase in activity and 2.1-fold increase in basal tension. Pretreatment of muscle strips with tetrodotoxin (1 μmol L−1) did not block the AR-C-induced response ( n = 5). In vivo, AR-C (30 μmol kg−1, i.v.) increased gallbladder contraction frequency ( P < 0.05; n = 8). These data suggest that iNOS is continually expressed in the normal gallbladder, which presumably releases low levels of nitric oxide and in turn may modulate spontaneous gallbladder motility. AR-C may be a beneficial treatment for patients suffering from acute cholecystitis. [ABSTRACT FROM AUTHOR]

Published

2007

129. Conditional mutant mice using tetracycline-controlled gene expression system in the brain

Author

Aiba, Atsu and Nakao, Harumi

Subjects

*GENE expression, *GENETIC regulation, *GENETICS, *GENETIC disorders

Abstract

Abstract: Generation of knockout mice with targeted mutations in desired genes is one of the most important technologies available for determining the functions of gene products in the brain. However, conventional knockout technology has limitations, such as when conventional knockout results in a lethal phenotype or when gene function at a certain developmental stage must be elucidated. To circumvent these limitations, a tetracycline-controlled gene expression system has been exploited to generate conditional mutant mice in which expression of desired genes can be switched on or off by oral administration of tetracycline derivatives. This up-date article introduces conditional mutant mice obtained using the tetracycline-controlled gene expression system, and presents several examples including our versatile mouse line, the mGluR1 conditional knockout mouse. [Copyright &y& Elsevier]

Published

2007

130. Inducible and reversible suppression of Npm1 gene expression using stably integrated small interfering RNA vector in mouse embryonic stem cells

Author

Wang, Bei Bei, Lu, Rui, Wang, Wei Cheng, and Jin, Ying

Subjects

*RNA, *CELL proliferation, *CELL division, *MOBILE genetic elements

Abstract

Abstract: The tetracycline (Tc)-inducible small interference RNA (siRNA) is a powerful tool for studying gene function in mammalian cells. However, the system is infrequently utilized in embryonic stem (ES) cells. Here, we present the first application of the Tc-inducible, stably integrated plasmid-based siRNA system in mouse ES cells to down-regulate expression of Npm1, an essential gene for embryonic development. The physiological role of Npm1 in ES cells has not been defined. Our data show that the knock-down of Npm1 expression by this siRNA system was not only highly efficient, but also Tc- dose- and induction time-dependent. Particularly, the down-regulation of Npm1 expression was reversible. Importantly, suppression of Npm1 expression in ES cells resulted in reduced cell proliferation. Taken together, this system allows for studying gene function in a highly controlled manner, otherwise difficult to achieve in ES cells. Moreover, our results demonstrate that Npm1 is essential for ES cell proliferation. [Copyright &y& Elsevier]

Published

2006

131. Allele-specific RNAi selectively silences mutant SOD1 and achieves significant therapeutic benefit in vivo

Author

Xia, Xugang, Zhou, Hongxia, Huang, Yong, and Xu, Zuoshang

Subjects

*NEURODEGENERATION, *TRANSGENIC mice, *AMYOTROPHIC lateral sclerosis, *SUPEROXIDES

Abstract

Abstract: RNA interference (RNAi) has the potential to treat diseases caused by dominant, gain-of-function type of gene mutations. In these diseases, one allele is mutated and produces a toxic protein, whereas the other allele is normal and performs vital functions. One challenge in the treatment is to specifically inhibit the mutant allele toxicity while maintaining the normal allele function. To test allele-specific silencing in vivo, we made transgenic mice that express an shRNA against mutant Cu, Zn superoxide dismutase gene (SOD1G93A), which causes amyotrophic lateral sclerosis (ALS) by a gain of an unknown toxic property. By crossing this transgenic line with mice that express SOD1G93A and mice that express wild-type human SOD1, we found that this shRNA specifically silences the mutant, but not the wild-type SOD1. The silencing of the mutant significantly delayed ALS onset and extended survival. Thus, RNAi can achieve allele-specific silencing and therapeutic benefit in vivo. [Copyright &y& Elsevier]

Published

2006

132. Production of human vitronectin in Nicotiana benthamiana using the INPACT hyperexpression platform

Author

Mark D. Harrison, James L. Dale, Robert M. Harding, Robyn Lloyd, Manuel R. Plan, Maiko Kato, Benjamin Dugdale, Terry Walsh, and Pradeep C. Deo

Subjects

0106 biological sciences, 0301 basic medicine, biopharming, Nicotiana benthamiana, INPACT, Plant Science, Biology, 01 natural sciences, 03 medical and health sciences, Tissue culture, Gene Expression Regulation, Plant, inducible, Tobacco, Humans, Vitronectin, Cell adhesion, Research Articles, Activator (genetics), Cell adhesion molecule, food and beverages, biology.organism_classification, Plants, Genetically Modified, Molecular biology, 030104 developmental biology, biology.protein, Expression cassette, Tomato bushy stunt virus, transgene expression, Agronomy and Crop Science, 010606 plant biology & botany, Biotechnology, Research Article

Abstract

Summary Human vitronectin (hVN) is a glycoprotein that functions as a cell adhesion molecule and a regulator of coagulation in blood plasma and the extracellular matrix. In vitro, hVN is added to serum‐free media in order to promote the adhesion of animal cells to tissue culture surfaces and the proliferation of undifferentiated stem cells. Here, we report the production of hVN in Nicotiana benthamiana using the inducible In Plant ACTivation (INPACT) hyperexpression platform. N. benthamiana plants were transformed with an INPACT expression cassette encoding hVN, and both the Tobacco yellow dwarf virus Rep/RepA activator and Tomato bushy stunt virus p19 gene under the transcriptional control of the ethanol‐inducible AlcR:alcA gene switch. hVN expression was maximal 4–5 days postactivation of the INPACT platform with a dilute ethanol solution, and crude yields of the recombinant protein reached a maximum of 643 ± 78 mg/kg fresh weight. A three‐stage purification protocol was developed using heparin and polyhistidine tag affinity binding and size exclusion filtration, resulting in a plant‐made hVN product of >90% purity. Storage conditions for plant‐made hVN were identified that maximized the capacity of the recombinant protein to promote cell adhesion. Critically, plant‐made hVN was shown to be functionally equivalent to commercial, plasma‐derived hVN at promoting one‐half maximal attachment of murine fibroblast cells (BALB‐C/3T3) in serum‐free medium at

Published

2017

133. Heat-inducible amplifier vector for high-level expression of granulocyte-macrophage colony-stimulating factor.

Author

Dammeyer, Pascal, Jaramillo, Melba C., Pipes, Brian L., Badowski, Michael S., Tsang, Tom C., and Harris, David T.

Subjects

*GRANULOCYTES, *MACROPHAGES, *CYTOKINES, *IMMUNOTHERAPY, *FEVER, *MELANOMA

Abstract

Purpose : In cytokine immunotherapy of cancer it is critical to deliver sufficiently high local cytokine concentrations in order to reach the therapeutic threshold needed for clinical efficacy. Simultaneously, for optimal clinical safety adverse effects caused by high systemic cytokine levels must be minimized. One of the most promising anti-cancer therapeutic cytokines, granulocyte-macrophage colony-stimulating factor (GM-CSF), has elicited anti-tumour immune responses in animal studies and clinical trials. However, the clinical efficacy has been limited, with local GM-CSF levels being therapeutically insufficient and systemic toxicity being a limiting factor. Methods : To address these problems we have developed a novel GM-CSF expression vector, pAD-HotAmp-GM-CSF, which can provide high levels of GM-CSF expression, and induction of cytokine expression to limited tissue areas. This expression system combines inducible and amplifying elements in a single multi-genic construct. The first transcriptional unit contains the inducible element, the heat shock protein 70B (HSP70B) promoter that regulates expression of the transcription-activating factor tat. Results : Upon the binding of tat to the second promoter, the HIV2 long terminal repeat amplifies downstream gene expression of the therapeutic cytokine GM-CSF. Moderate hyperthermia at 42°C for 30&ThickSpace;min induced GM-CSF expression in pAD-HotAmp-GM-CSF that was over 2.5- and 2.8-fold higher than levels reached with HSP70B promoter alone and the prototypical human cytomegalovirus promoter. Conclusions : Thus, the inducible amplifier vector, pAD-HotAmp-GM-CSF, represents a novel system for regulated and enhanced GM-CSF expression, which enables both greater efficacy and safety in cytokine immunotherapy of cancer. [ABSTRACT FROM AUTHOR]

Published

2006

134. Jun signalling in the epidermis: From developmental defects to psoriasis and skin tumors

Author

Zenz, Rainer and Wagner, Erwin F.

Subjects

*EPIDERMAL growth factor, *PSORIASIS, *SKIN tumors, *PROTEIN kinases

Abstract

Abstract: The Jun proteins Jun, JunB and JunD are core members of activator protein-1 (AP-1), a dimeric transcription factor complex consisting of homo- and heterodimers of the Jun, Fos, activating transcription factor (ATF) and musculoaponeurotic fibrosarcoma (Maf) families. Growth factors, hormones and a variety of environmental stresses activate mitogen activated protein kinase (MAPK) cascades that enhance Jun/AP-1 activity, e.g. through phosphorylation thereby regulating cell proliferation, differentiation, transformation and/or apoptosis. Embryonic lethality of various AP-1 knock-outs, e.g. for Jun, JunB, Fra-1 and Fra-2 largely prevented functional studies in vivo. Therefore, conditional knock-out strategies, in particular for the epidermis, have become an important model to study the regulation and function of AP-1 subunits in physiological and pathological processes in vivo. Jun is regarded as a positive regulator of keratinocyte proliferation/differentiation during development and in skin cancer through its direct transcriptional effect on epidermal growth factor receptor (EGFR) expression. In contrast, JunB can antagonize proliferation of keratinocytes and hematopoietic stem cells. Furthermore, it has been demonstrated in patient''s samples and an inducible mouse model that down-regulation of JunB/AP-1 in keratinocytes is one initiating event in the aetiology of psoriasis which is characterized by increased cell proliferation and deregulated cytokine expression. [Copyright &y& Elsevier]

Published

2006

135. Conditional and inducible gene recombineering in the mouse inner ear

Author

Tian, Yong, James, Sally, Zuo, Jian, Fritzsch, Bernd, and Beisel, Kirk W.

Subjects

*TRANSGENIC mice, *GENETIC engineering, *TRANSGENIC organisms, *INNER ear, *TAMOXIFEN, *TETRACYCLINE, *TRANSGENES

Abstract

Abstract: Genetically engineered mice have greatly improved our understanding of gene functions and disease mechanisms. Nevertheless, the traditional knock-out approach has limitations in the overall viability of mutants. The application of the Cre/loxP system in the inner ear can help bypass this difficulty by generation of conditional gene recombineering. However, to do so requires an expression system that allows ear-specific temporally inducible, gene abrogation of one or more of the increasingly available floxed genes. To date, three approaches have been successfully used to create murine inner ear-specific Cre lines: conventional transgenesis, BAC transgenesis, and gene knock-in. Unfortunately, timing of conditional Cre activity does not extend beyond the regulatory range of the gene controlling Cre expression. Rectification of this problem requires the generation of tamoxifen or tetracycline inducible systems in the inner ear. Examination of integrase expression at different loci will facilitate studies on the expression of exogenous transgenes. These genetic applications for the mouse genome will dramatically advance in vivo gene function studies. [Copyright &y& Elsevier]

Published

2006

136. Inactivation of the putative tetracycline resistance gene HP1165 in Helicobacter pylori led to loss of inducible tetracycline resistance.

Author

Yuhuan Li and Dannelly, H.

Subjects

*TETRACYCLINE, *GENES, *ANTIBIOTICS, *DRUG resistance, *HELICOBACTER pylori infections, *GENETIC mutation

Abstract

Tetracycline has been used with other antibiotics in treatment of Helicobacter pylori infection. However, tetracycline resistance has developed in H. pylori clinical isolates, rendering treatment failure. Mutations in 16S rRNA genes have been reported to mediate tetracycline resistance in some isolates. The diversity of tetracycline resistance cases suggests multiple genes are involved. HP1165, a putative tetracycline resistance gene in H. pylori 26695, displays 49.8% identity to the tetracycline efflux gene tetA (P) from Clostridium perfringens. To determine the function of the HP1165 gene in H. pylori, the tetracycline resistance phenotype was investigated, transcription of HP1165 was examined by RT-PCR, and a ΔHP1165 mutant was generated by insertion of the pBCα3 plasmid. The results showed that strains harboring HP1165 were induced to intermediate level resistance in the laboratory (minimum inhibitory concentration=4–6 μg/ml). No mutation was found at or near the tetracycline binding sites of the 16S rRNA gene. The gene was transcribed both in the induced tetracycline resistant and wild type strains, indicating translational or posttranslational control of gene function. Mutation of HP1165 gene resulted in increased tetracycline susceptibility and loss of inducible tetracycline resistance, suggesting that the HP1165 gene is involved in the inducible tetracycline resistance in H. pylori. [ABSTRACT FROM AUTHOR]

Published

2006

137. Inducible nitric oxide synthase inhibitors abolished histological protection by late ischemic preconditioning in rat retina

Author

Sakamoto, Kenji, Yonoki, Yuzuru, Kubota, Yuko, Kuwagata, Mayumi, Saito, Maki, Nakahara, Tsutomu, and Ishii, Kunio

Subjects

*NITRIC-oxide synthases, *RETINAL blood vessel diseases, *INTRAOCULAR pressure, *ANIMAL models in research, *RESEARCH methodology

Abstract

Abstract: Brief ischemia was reported to protect retinal cells against injury induced by subsequent ischemia-reperfusion with de novo protein synthesis, and this phenomenon is known as late ischemic preconditioning. The aims of the present study were to determine whether nitric oxide synthase (NOS) was involved in the mechanism of late ischemic preconditioning in rat retina using pharmacological tools. Under anesthesia with pentobarbital sodium, male Sprague-Dawley rats were subjected to 60min of retinal ischemia by raising intraocular pressure to 130mmHg. Ischemic preconditioning was achieved by applying 5min of ischemia 24hrs before 60min of ischemia. Retinal sections sliced into 5μm thick were examined 7 days after ischemia. Additional groups of rats received NG-nitro-l-arginine and NG-monomethyl-l-arginin, non-selective NO synthase inhibitors, 7-nitroindazole, a neuronal NOS inhibitor, and aminoguanidine and l-N6-(1-iminoethyl) lysine, inducible NO synthase (iNOS) inhibitors before preconditioning, and were subjected to 60min of ischemia. In the non-preconditioned group, cell loss in the ganglion cell layer and thinning of the inner plexiform and inner nuclear layer were observed 7 days after 60min of ischemia. Ischemic preconditioning for 5min completely protected against the histological damage induced by 60min of ischemia applied 24hrs thereafter. Treatment of rats with aminoguanidine and l-N6-(1-iminoethyl) lysine, but not NG-nitro-l-arginine, NG-monomethyl-l-arginine or 7-nitroindazole, wiped off the protective effect of ischemic preconditioning. The inhibitory effect of aminoguanidine was abolished by l-arginine, but not d-arginine. The results in the present study suggest that NO synthesized by iNOS is involved in the histological protection by late ischemic preconditioning in rat retina. [Copyright &y& Elsevier]

Published

2006

138. Use of an in vitro Model and Yeast Two-Hybrid System to Investigate the Pathogenesis of Hepatitis C.

Author

Seng Gee Lim, Yee Joo Tan, Phuay Yee Goh, Siew Pheng Lim, and Wan Jin Hong

Subjects

*HEPATITIS C virus, *CYTOLOGY, *SERUM, *PATIENTS

Abstract

Fifteen years after the discovery of hepatitis C virus (HCV) in 1989, much remains to be learnt about the cell biology of this virus. Using the serum from a patient containing HCV RNA in high titer as a source, a Singapore strain of genotype 1b was recovered and characterized. This full-length HCV genome was then constructed into a tetracycline-inducible vector using the pSTAR plasmid. Transfection of hepatoma cell lines with this HCV genome under tetracycline induction indicated that chemokines (RANTES and monocyte chemoattractant protein-1) were upregulated, possibly contributing to the induction of immune responses. Using the yeast two-hybrid system to discover protein-protein interactions, nonstructural region NS3 was found to interact with itself, forming a dimer that increased helicase activity but was not essential for its activity, thereby disqualifying it as a suitable target of drug actions. The significance of the interaction between core and NS5A is unclear, and the cleavage of NS5A is related to the development of apoptosis. However, the interaction of p68 and NS56B appears to be important because the knockdown of p68 reduced the viral replication. Finally, a new cell model using chimeric CD81 linked to the cytoplasmic domain of either a low-density lipoprotein receptor or a transferrin receptor led to productive infection of HCV that had been recovered from infected serum. These studies allow us to examine the pathogenesis of HCV infection in more detail. Copyright © 2006 S. Karger AG, Basel [ABSTRACT FROM AUTHOR]

Published

2006

139. A stable, inducible, dose-responsive ODC overexpression system in human cell lines

Author

Wilson, Shannon M., Hawel, Leo, Pastorian, Kirk E., and Byus, Craig V.

Subjects

*CELL lines, *CELL culture, *MESSENGER RNA, *RNA

Abstract

Abstract: ODC is a labile protein subject to rapid turnover, and a conditional expression system providing long-term overexpression may be helpful in further understanding the biochemical properties of this enzyme and elucidating aspects of the polyamine biosynthetic pathway that have otherwise been difficult to study. HEK293 and LNCaP cell lines were engineered to stably and inducibly overexpress ODC using a Tet-on inducible construct. Clones from both cell lines were characterized by evaluating ODC mRNA expression, ODC activity, intracellular and extracellular polyamine levels, SSAT activity and growth kinetics. The ODC-inducible cell lines were time- and dose-responsive providing a mechanism to increase ODC and putrescine accumulation to a desired level in a flexible and controllable manner. The findings demonstrate that LNCaP ODC overexpressing cells maintained over a 100-fold increase in ODC activity and over a 10-fold increase in intracellular putrescine after 6 h. ODC induction at the highest levels was accompanied by a slight decline in intracellular spermidine and spermine levels and this observation was supported by the finding that SSAT activity was induced over 40-fold under these conditions. Growth rate remained unaffected following at least 12 h of ODC overexpression. Similar results were observed in the HEK293 ODC overexpressing cells. [Copyright &y& Elsevier]

Published

2005

140. Construction of an inducible expression shuttle vector for Laribacter hongkongensis, a novel bacterium associated with gastroenteritis

Author

Woo, Patrick C.Y., Ma, Shirley S.L., Teng, Jade L.L., Li, Maria W.S., Kao, Richard Y.T., Lau, Susanna K.P., and Yuen, Kwok-yung

Subjects

*ESCHERICHIA coli, *GASTROENTERITIS, *ESCHERICHIA, *GASTROINTESTINAL diseases

Abstract

Abstract: An Escherichia coli–Laribacter hongkongensis shuttle vector (pPW380) was constructed by ligating the 4701-bp EcoRI digested fragment of pHLHK8 to EcoRI digested pBK-CMV. An E. coli–L. hongkongensis inducible expression shuttle vector was further constructed by ligating a 2105-bp fragment that contains the tetracycline repressor and tetracycline-inducible promoter region of pALC2084 to the 8897-bp fragment of pPW380, deletion of the green fluorescent protein gene, and insertion of a multiple cloning site. This inducible expression system was able to express two commonly used reporter genes, the green fluorescent protein gene and the glutathione S-transferase gene, efficiently in E. coli and L. hongkongensis. [Copyright &y& Elsevier]

Published

2005

141. Pitavastatin Prevents Bacterial Translocation after Nonpulsatile/Low-Pressure Blood Flow in Early Atherosclerotic Rat: Inhibition of Small Intestine Inducible Nitric Oxide Synthase.

Author

Tsunooka, N., Nakagawa, H., Doi, T., Yukumi, S., Sato, K., Horiuchi, A., Miyauchi, K., Watanabe, Y., Imagawa, H., and Kawachi, K.

Subjects

*ATHEROSCLEROSIS, *CARDIOPULMONARY bypass, *INTESTINAL mucosa, *BLOOD flow, *HYPOTENSION, *RATS, *STATINS (Cardiovascular agents), *NITRIC oxide

Abstract

Background: Cardiopulmonary bypass decreases intestinal mucosal blood flow because of nonpulsatile and low-pressure blood flow resulting in bacterial translocation (BT) and atherosclerosis also has peripheral blood flow deficiency. The risk of nonpulsatile and low-pressure blood flow for atherosclerotic animals and the effect of statin administration, which has pleiotropic effects, were studied. Methods: Wistar rats were divided into four groups: group N (normal diet), group C (high-cholesterol diet), group S (group C plus pitavastatin therapy), and group I [group C plus inducible nitric oxide (iNOS) inhibitor therapy]. First of all, vascular responses were measured. Then the rats underwent nonpulsatile/low-pressure blood flow in the intestine, and the serum peptidoglycan concentration as a parameter of BT, the small intestinal PO2 ratio (intestinal PO2/PaO2) as a parameter of mucosal blood flow, and NO concentrations were measured before surgery (T0), at the end of 90 min of stenosis (T1), and 90 min after the release of stenosis (T2). Immunostaining for nitrotyrosine was also performed at T2. Results: Group C had vascular endothelial dysfunction without histological changes, which indicated early atherosclerosis. The serum peptidoglycan concentration increased significantly at T2 only in group C. The intestinal PO2 ratio was decreased at T1 in all the groups, and retuned to baseline at T2 in group N and group S, but not in group C or group I. Jejunal NO only in group C was significantly higher at all time points and ileal NO production at T1 and T2. There tended to be a positive stain for nitrotyrosine along the mucosal epithelium in group C. Conclusion: In the setting of early atherosclerosis, intestinal blood flow does not only improve after nonpulsatile/low-pressure blood flow but causes BT because of a large amount of NO from high enzymatic intestinal iNOS activity, and pitavastatin treatment can prevent BT by improving both issues. [ABSTRACT FROM AUTHOR]

Published

2005

142. Constitutive activity of human angiotensin II type-1 receptors by Gq overexpression

Author

Scragg, Jason L., Warburton, Philip, Ball, Stephen G., and Balmforth, Anthony J.

Subjects

*ANGIOTENSINS, *OLIGOPEPTIDES, *CELL culture, *G proteins

Abstract

Abstract: We have developed an inducible HEK293/Tet-On cell line that transiently expresses both FLAG-tagged human angiotensin II type-I receptors (FLAG-hAT1R) and Gqα G protein subunits in response to doxycycline. High and tightly regulated levels of FLAG-hAT1R (740±57fmol/mg protein) and Gqα (36-fold increase compared with non-induced cells) overexpression were consistently achieved. We investigated the possibility of using an inducible system to increase the proportion of constitutively active wild-type FLAG-hAT1Rs by overexpressing Gqα. Following doxycycline treatment, we observed no significant change in the apparent binding affinity or potency (coupling efficiency) of angiotensin II, though significant increases in the intrinsic activity of several partial agonists were observed, indicative of constitutive activity. DUP753 (10μM), a suggested inverse agonist, did not inhibit the enhanced level of basal (agonist-independent) activity. The data suggest that the resting equilibrium of hAT1 receptors between the inactive (R) and active (R*) forms is predominantly weighted towards the inactive conformation. [Copyright &y& Elsevier]

Published

2005

143. Influence of 5′ sequences on expression of the Tet repressor in Giardia lamblia

Author

Sun, Chin-Hung, Su, Li-Hsin, and Gillin, Frances D.

Subjects

*GIARDIA lamblia, *GENE expression, *ESCHERICHIA coli, *NUCLEIC acids

Abstract

Abstract: Gene expression is poorly understood in Giardia lamblia. Previously we utilized the Escherichia coli tetracycline regulatory elements to develop a giardial-inducible gene expression system. In this study, we tested the hypothesis that regions flanking the tet repressor (tet R) may influence its expression and affect inducibility of the regulatory system. We found that addition of a 6-His tag or nuclear localization signal (NLS) at the N- but not C-terminus of tet R, increased the induction ratios >100-fold. A non-specific sequence also increased the induction ratio. Fusing NLS at the N-terminus, also led to exclusively nuclear tet R localization. Changing the promoter from gdh or α-giardin to α2-tubulin increased the induction ratio slightly. Tet R expression at both RNA and protein levels correlated with repression efficiency, indicating that coding sequences of the 6-His tag or NLS may contribute to transcriptional activation of the exotic tet R gene in Giardia. In addition, we found that the tet R system mediated gene repression and induction during encystation. Previous studies used an artificial reporter gene. In this study, we were able to induce overexpression of epitope-tagged cyst wall protein 1 (CWP1) in vegetatively growing Giardia trophozoites. Moreover, we could repress or induce expression of exogenous CWP1 in encysting cells. Taken together, our data suggest that expression of tet R in Giardia is complex and can be strongly influenced by additional sequences, especially at its N-terminus. This system provides insights into expression of an alien gene and can be exploited to regulate gene expression and study important functions in G. lamblia. [Copyright &y& Elsevier]

Published

2005

144. High-level expression of a novel amine-synthesizing enzyme, N-substituted formamide deformylase, in Streptomyces with a strong protein expression system

Author

Fukatsu, Hiroshi, Herai, Sachio, Hashimoto, Yoshiteru, Maseda, Hideaki, Higashibata, Hiroki, and Kobayashi, Michihiko

Subjects

*ESCHERICHIA coli, *GENE expression, *GENETIC regulation, *ENTEROBACTERIACEAE

Abstract

Abstract: N-substituted formamide deformylase (NfdA) from Arthrobacter pascens F164 is a novel deformylase involved in the metabolism of isonitriles. The enzyme catalyzes the deformylation of an N-substituted formamide, which is produced from the corresponding isonitrile, to yield the corresponding amine and formate. The nfdA gene from A. pascens F164 was cloned into different types of expression vectors for Escherichia coli and Streptomyces strains. Expression in E. coli resulted in the accumulation of an insoluble protein. However, Streptomyces strains transformed with a PnitA-NitR system, which we very recently developed as a regulatory gene expression system for streptomycetes, allowed the heterologous overproduction of NfdA in an active form. When Streptomyces lividans TK24 transformed with pSH19-nfdA was cultured under the optimum conditions, the NfdA activity of the cell-free extract amounted to 8.5U/mg, which was 29-fold higher than that of A. pascens F164. The enzyme also comprised ≈20% of the total extractable cellular protein. The recombinant enzyme was purified to homogeneity and characterized. The expression system established here will allow structural analysis and mutagenesis studies of NfdA. [Copyright &y& Elsevier]

Published

2005

145. eNOS, nNOS, cGMP and protein kinase G mediate the inhibitory effect of pancreastatin, a chromogranin A-derived peptide, on growth and proliferation of hepatoma cells

Author

Díaz-Troya, Sandra, Najib, Souad, and fSánchez-Margalet, Víctor

Subjects

*PROTEIN kinases, *LIVER tumors, *NITROGEN compounds, *PROTEIN kinase C

Abstract

Abstract: Pancreastatin (PST), a chromogranin A-derived peptide, has an anti-insulin metabolic effect and inhibits growth and proliferation by producing nitric oxide (NO) in HTC rat hepatoma cells. When NO production is blocked, a proliferative effect prevails due to the activation a Gαq/11-phospholipase C-β (PLC-β) pathway, which leads to an increase in [Ca2+]i, protein kinase C (PKC) and mitogen-activated protein kinase (MAPK) activation. The aim of the present study was to investigate the NO synthase (NOS) isoform that mediates these effects of PST on HTC hepatoma cells and the possible roles of cyclic GMP (cGMP) and cGMP-dependent protein kinase. DNA and protein synthesis in response to PST were measured as [3H]-thymidine and [3H]-leucine incorporation in the presence of various pharmacological inhibitors: N-monomethyl-l-arginine (NMLA, nonspecific NOS inhibitor), l-NIO (endothelial nitric oxide synthase (eNOS) inhibitor), espermidine (neuronal nitric oxide synthase (nNOS) inhibitor), LY83583 (guanylyl cyclase inhibitor), and KT5823 (protein kinase G inhibitor, (PKG)). l-NIO, similarly to NMLA, reverted the inhibitory effect of PST on hepatoma cell into a stimulatory effect on growth and proliferation. Nevertheless, espermidine also prevented the inhibitory effect of PST, but there was no stimulation of growth and proliferation. When guanylyl cyclase activity was blocked, there was again a reversion of the inhibitory effect into a stimulatory action, suggesting that the effect of NO was mediated by the production of cGMP. PKG inhibition prevented the inhibitory effect of PST, but there was no stimulatory effect. Therefore, the inhibitory effect of PST on growth and proliferation of hepatoma cells may be mainly mediated by eNOS activation. In turn, the effect of NO may be mediated by cGMP, whereas other pathways in addition to PKG activation seem to mediate the inhibition of DNA and protein synthesis by PST in HTC hepatoma cells. [Copyright &y& Elsevier]

Published

2005

146. Analysis and characterization of the transcriptional unit of a new Mytilus galloprovincialis (Mollusca: Bivalvia) hsp70 gene.

Author

Kourtidis, Antonis and Scouras, Zacharias G.

Subjects

*MYTILUS galloprovincialis, *MYTILUS, *AMINO acid analysis, *AMINO acid sequence, *CALIFORNIA mussel, *MYTILUS edulis

Abstract

We isolated, analysed and characterized the transcriptional unit of an hsp70 gene of Mytilus galloprovincialis (Mollusca: Bivalvia). Sequence analysis of a total of 3653?bp, revealed a 1914?bp ORF encoding for a 637-amino acid polypeptide that exhibits all the characteristic signatures of the cytoplasmic members of the HSP70 family. The ORF is not interrupted by introns and its 5'-flanking region contains five putative heat shock elements (HSEs), both indicating for an inducible hsp70 gene. Furthermore, nucleotide and amino acid sequence alignments with HSP70 genes from several molluscan and non-molluscan species confirmed that the newly isolated gene, the first complete in the genus Mytilus and in the Mollusca phylum, is a cytoplasmic and inducible hsp70 gene. [ABSTRACT FROM AUTHOR]

Published

2005

147. Bactericidal activity of quinupristin-dalfopristin against strains of Staphylococcus aureus with the MLSB phenotype of resistance according to the erm gene type

Author

Clarebout, G., Nativelle, E., Bozdogan, B., Villers, C., and Leclercq, R.

Subjects

*STREPTOGRAMINS, *MICROCOCCACEAE, *GENETIC research, *QUINUPRISTIN

Abstract

The bactericidal activity of quinupristin-dalfopristin was assessed by time-kill experiments against Staphylococcus aureus strains with characterized phenotypes and genotypes of MLSB resistance. A set of laboratory strains composed of isogenic pairs of S. aureus RN4220 derivatives containing or not the erm(A), erm(B) or erm(C) genes constitutively expressed and of 13 clinical isolates containing these genes inducibly or constitutively expressed were studied. Three of the clinical isolates with erm(B) or erm(A) genes had an unusual inducible MLSB cross resistance. The early bactericidal activity of quinupristin-dalfopristin was altered against strains expressing constitutive quinupristin resistance regardless of the erm(A), erm(B) or erm(C) type of gene. We conclude that the bactericidal activity of quinupristin-dalfopristin against staphylococci was dependent on the activity of quinupristin rather than on the erm genotype of the strain. [Copyright &y& Elsevier]

Published

2004

148. Molecular cloning and characterization of canine ICOS

Author

Lee, Je-Hwan, Joo, Young-Don, Yim, Daesong, Lee, Richard, Ostrander, Elaine A., Loretz, Carol, Little, Marie-Térèse, Storb, Rainer, and Kuhr, Christian S.

Subjects

*GENETIC engineering, *MOLECULAR cloning, *HEMATOPOIETIC stem cells, *CELLULAR therapy, *NUCLEIC acids

Abstract

Inducible costimulatory receptor (ICOS) is one recently identified member of the CD28 family of costimulatory molecules. Evidence suggests ICOS functions as a critical immune regulator and, to evaluate these effects, we employed the canine model system that has been used to develop strategies currently in clinical use for hematopoietic stem cell transplantation. To investigate the effects of blocking the ICOS pathway in the canine hematopoietic cell transplantation model, we tested existing murine and human reagents and cloned the full length of the open reading frame of canine ICOS cDNA to allow the development of reagents specific for the canine ICOS. Canine ICOS contains a major open reading frame of 624 nucleotides, encoding a protein of 208 amino acids, and localizes to chromosome 37. Canine ICOS shares 79% sequence identity with human ICOS, 70% with mouse, and 69% with rat. Canine ICOS expression is limited to stimulated PBMC. [Copyright &y& Elsevier]

Published

2004

149. Transactivator and Structurally Optimized Inducible Lentiviral Vectors

Author

Haack, Karin, Cockrell, Adam S., Ma, Hong, Israeli, David, Ho, Steffan N., McCown, Thomas J., and Kafri, Tal

Subjects

*LENTIVIRUSES, *BRAIN, *GENE therapy, *THERAPEUTICS

Abstract

Lentiviral vectors offer well-recognized advantages as a gene delivery system both for the analysis of gene function and as a vehicle for gene therapy. In the present study optimized HIV-1-based vector systems that display efficient doxycycline (Dox)-dependent transgene expression in vitro and in vivo have been developed through the modification of factors that contribute to basal activity levels. Dissection of HIV-1 vectors harboring a tTA-dependent transgene expression cassette revealed several mechanisms that account for Dox-independent transgene expression, including those mediated by an internal CMV promoter, as well as a potential contribution from fusion proteins generated by translational readthrough. A precipitous reduction in basal activity levels was accomplished by separating the transactivator and the transgene cassettes into a binary vector system and by relocating the inducible promoter to the U3 region of the LTR. In addition, substituting the VP16 portion of tTA with the human p65 transactivating domain improved Dox-dependent transgene expression in a number of cell types. Optimizing HIV-1-based vectors culminated in a “toolbox” of vectors suitable for transgene delivery in vitro and in vivo, as conveyed by our ability to control the Dox-dependent differentiation of embryonic fibroblasts into muscle cells in vitro and transgene expression in rat brains. [Copyright &y& Elsevier]

Published

2004

150. Gene-targeting technologies for the study of neurological disorders.

Author

Beglopoulos, Vassilios and Shen, Jie

Abstract

Studies using genetic manipulations have proven invaluable in the research of neurological disorders. In the forefront of these approaches is the knockout technology that engineers a targeted gene mutation in mice resulting in inactivation of gene expression. In many cases, important roles of a particular gene in embryonic development have precluded the in vivo study of its function in the adult brain, which is usually the most relevant experimental context for the study of neurological disorders. The conditional knockout technology has provided a tool to overcome this restriction and has been used successfully to generate viable mouse models with gene inactivation patterns in certain regions or cell types of the postnatal brain. This review first describes the methodology of gene targeting in mice, detailing the aspects of designing a targeting vector, introducing it into embryonic stem cells in culture and screening for correct recombination events, and generating chimeric and null mutant mice from the positive clones. It then discusses the special issues and considerations for the generation of conditional knock-out mice, including a section about approaches for inducible gene inactivation in the brain and some of their applications. An overview of gene-targeted mouse models that have been used in the study of several neurological disorders, including Alzheimer’s disease, Parkinson’s disease, Huntington’s disease, seizure disorders, and schizophrenia, is also presented. The importance of the results obtained by these models for the understanding of the pathogenic mechanism underlying the disorders is discussed. [ABSTRACT FROM AUTHOR]

Published

2004