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2. The C. elegans maternal-effect gene clk-2 is essential for embryonic development, encodes a protein homologous to yeast Tel2p and affects telomere length.

Author

Bénard, C, McCright, B, Zhang, Y, Felkai, S, Lakowski, B, and Hekimi, S

Abstract

The Caenorhabditis elegans maternal-effect clk genes are involved in the temporal control of development and behavior. We report the genetic and molecular characterization of clk-2. A temperature-sensitive mutation in the gene clk-2 affects embryonic and post-embryonic development, reproduction, and rhythmic behaviors. Yet, virtually all phenotypes are fully maternally rescued. Embryonic development strictly requires the activity of maternal clk-2 during a narrow time window between oocyte maturation and the two- to four-cell embryonic stage. Positional cloning of clk-2 reveals that it encodes a protein homologous to S. cerevisiae Tel2p. In yeast, the gene TEL2 regulates telomere length and participates in gene silencing at subtelomeric regions. In C. elegans, clk-2 mutants have elongated telomeres, and clk-2 overexpression can lead to telomere shortening. Tel2p has been reported to bind to telomeric DNA repeats in vitro. However, we find that a functional CLK-2::GFP fusion protein is cytoplasmic in worms. We discuss how the phenotype of clk-2 mutants could be the result of altered patterns of gene expression.

Published
2001

3. Mouse CLK-1 is imported into mitochondria by an unusual process that requires a leader sequence but no membrane potential.

Author

Jiang, N, Levavasseur, F, McCright, B, Shoubridge, E A, and Hekimi, S

Abstract

clk-1 has been identified and characterized in the nematode Caenorhabditis elegans as a gene that affects the rates, regularity, and synchrony of physiological processes. The CLK-1 protein is mitochondrial and is required for ubiquinone biosynthesis in yeast and in worms, but its biochemical function remains unclear. We have studied the expression of murine mclk1 in a variety of tissues, and we find that the pattern of mclk1 mRNA accumulation closely resembles that of mitochondrial genes involved in oxidative phosphorylation. The pattern of protein accumulation, however, is sharply distinct in some tissues; mCLK1 appears relatively enriched in the gut and depleted in the nervous tissue. We also show that mCLK1 is synthesized as a preprotein that is imported into the mitochondrial matrix, where a leader sequence is cleaved off and the protein becomes loosely associated with the inner membrane. However, in contrast to all known mitochondrial proteins that contain a cleavable pre-sequence, the import of mCLK1 does not require a mitochondrial membrane potential.

Published
2001
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4. Identification of a new family of protein phosphatase 2A regulatory subunits.

Author

McCright, B and Virshup, D M

Abstract

Protein phosphatase 2A (PP2A) is a major intracellular protein phosphatase that regulates multiple aspects of cell growth and metabolism. The ability of this widely distributed heterotrimeric enzyme to act on a diverse array of substrates is largely controlled by the nature of its regulatory B subunit. Only two gene families encoding endogenous B subunits have been cloned to date, although the existence of several additional regulatory subunits is likely. We have identified by two-hybrid interaction a new human gene family encoding PP2A B subunits. This family, denoted B56, contains three distinct genes, one of which is differentially spliced. B56 polypeptides co-immunoprecipitate with PP2A A and C subunits and with an okadaic acid-inhibitable, heparin-stimulated phosphatase activity. The three B56 family members are 70% identical to each other but share no obvious homology with previously identified B subunits. These phosphatase regulators are differentially expressed, with B56 alpha and B56 gamma highly expressed in heart and skeletal muscle and B56 beta highly expressed in brain. The identification of this novel phosphatase regulator gene family will facilitate future studies on the control of protein dephosphorylation and the role of PP2A in cellular function.

Published
1995

5. A new method to improve RF safety of implantable medical devices using inductive coupling at 3.0 T MRI.

Author

Park BS, Guag JW, Jeong H, Rajan SS, and McCright B

Subjects
Humans, Magnetic Fields, Phantoms, Imaging, Magnetic Resonance Imaging methods, Radio Waves, Prostheses and Implants, Electromagnetic Fields
Abstract

Objective: To enhance RF safety when implantable medical devices are located within the body coil but outside the imaging region by using a secondary resonator (SR) to reduce electric fields, the corresponding specific absorption rate (SAR), and temperature change during MRI., Materials and Methods: This study was conducted using numerical simulations with an American Society for Testing and Materials (ASTM) phantom and adult human models of Ella and Duke from Virtual Family Models, along with corresponding experimental results of temperature change obtained using the ASTM phantom. The circular SR was designed with an inner diameter of 150 mm and a width of 6 mm. Experimental measurements were carried out using a 3 T Medical Implant Test System (MITS) body coil, electromagnetic (EM) field mapping probes, and an ASTM phantom., Results: The magnitudes of B 1 (|B + (|B 1 were reduced by 15.2% and 5.85% within the volume of interest (VoI) of an ASTM phantom, when a SR that generates opposing electromagnetic fields was utilized. Likewise, the Δ|B + |) and SAR 1g were reduced by 15.2% and 5.85% within the volume of interest (VoI) of an ASTM phantom, when a SR that generates opposing electromagnetic fields was utilized. Likewise, the Δ|B 1 + | and ΔSAR 1g were reduced by up to 56.7% and 57.5% within the VoI of an Ella model containing a copper rod when an opposing SR was used., Conclusion: A novel method employing the designed SR, which generates opposing magnetic fields to partially shield a sample, has been proposed to mitigate the risk of induced-RF heating at the VoI through numerical simulations and corresponding experiments under various conditions at 3.0 T., (© 2023. This is a U.S. Government work and not under copyright protection in the US; foreign copyright protection may apply.)

Published
2023
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6. Growth arrest of PPP2R5C and PPP2R5D double knockout mice indicates a genetic interaction and conserved function for these PP2A B subunits.

Author

Dyson JJ, Abbasi F, Varadkar P, and McCright B

Abstract

Protein phosphatase 2A (PP2A) is a heterotrimeric phosphatase that controls a wide range of cellular functions. The catalytic activity and intracellular location of PP2A are modulated by its association with regulatory B subunits, including B56 proteins, which are encoded by five separate genes in humans and mice. The specific effects of each B56 protein on PP2A activity and function are largely unknown. As part of an effort to identify specific PP2A-B56 functions, we created knockout strains of B56β, B56δ, and B56ε using CRISPR/Cas9n. We found that none of the individual B56 genes are essential for mouse survival. However, mice that have both B56δ and B56γ inactivated (B56δγ-), arrest fetal development around Day E12. The hearts of B56δγ- mice have a single outflow vessel rather than having both an aorta and a pulmonary artery. Thus, there appears to be strong genetic interaction between B56δ and B56γ, and together they are necessary for heart development. Of note, both these proteins have been shown to localize to the nucleus and have the most related peptide sequences of the B56 family members. Our results suggest there are B56 subfamilies, which work in conjunction to regulate specific PP2A functions., Competing Interests: The authors have no conflict of interest to declare., (Published 2021. This article is a U.S. Government work and is in the public domain in the USA. FASEB BioAdvances published by Wiley Periodicals LLC on behalf of The Federation of American Societies for Experimental Biology.)

Published
2021
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7. Sensitivity and uniformity improvement of phased array MR images using inductive coupling and RF detuning circuits.

Author

Park BS, Rajan SS, and McCright B

Subjects
Animals, Equipment Design, Magnetic Fields, Mice, Phantoms, Imaging, Magnetic Resonance Imaging, Radio Waves
Abstract

Objective: To improve sensitivity and uniformity of MR images obtained using a phased array RF coil, an inductively coupled secondary resonator with RF detuning circuits at 300 MHz was designed., Materials and Methods: A secondary resonator having detuning circuits to turn off the resonator during the transmit mode was constructed. The secondary resonator was located at the opposite side of the four-channel phased array to improve sensitivity and uniformity of the acquired MR images. Numerical simulations along with phantom and in vivo experiments were conducted to evaluate the designed secondary resonator., Results: The numerical simulation results of |B 1 | in a transmit mode showed that magnetic field uniformity would be decreased with a secondary resonator having no detuning circuits because of unwanted interferences between the transmit birdcage coil and the secondary resonator. The standard deviation (SD) of |B + | was decreased 57% with a secondary resonator containing detuning circuits. The sensitivity and uniformity of |B 1 + | was decreased 57% with a secondary resonator containing detuning circuits. The sensitivity and uniformity of |B 1 - | in the receive mode using a four-channel phased array were improved with the secondary resonator. Phantom experiments using a uniform saline phantom had 20% improvement of the mean signal intensity and 50% decrease in the SD with the secondary resonator. Mice with excess adipose tissue were imaged to demonstrate the utility of the secondary resonator., Conclusion: The designed secondary resonator having detuning circuits improved sensitivity and uniformity of mouse MR images acquired using the four-channel phased array.

Published
2020
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8. Improvement of 19 F MR image uniformity in a mouse model of cellular therapy using inductive coupling.

Author

Park BS, Ma G, Koch WT, Rajan SS, Mastromanolis M, Lam J, Sung K, and McCright B

Subjects
Animals, Equipment Design, Fluorocarbons, Mice, Models, Theoretical, Phantoms, Imaging, Radio Waves, Signal-To-Noise Ratio, Cell Tracking methods, Fluorine chemistry, Fluorine-19 Magnetic Resonance Imaging, Magnetic Fields, Stem Cell Transplantation
Abstract

Objective: Improve 19 F magnetic resonance imaging uniformity of perfluorocarbon (PFC)-labeled cells by using a secondary inductive resonator tuned to 287 MHz to enhance the induced radio frequency (RF) magnetic field (B 1 ) at 7.05 T., Materials and Methods: Following Faraday's induction law, the sign of induced B 1 made by the secondary resonator can be changed depending on the tuning of the resonator. A secondary resonator located on the opposite side of the phantom of the 19 F surface coil can be shown to enhance or subtract the induced B 1 field, depending upon its tuning., Results: The numerical simulation results of rotating transmit B 1 magnitude (|B 1 + F images were compared without and with the secondary resonator. With the secondary resonator tuned to 287 MHz, improvements of |B 19 F images were compared without and with the secondary resonator. With the secondary resonator tuned to 287 MHz, improvements of |B 1 + | and 19 F image uniformity were demonstrated. The use of the secondary resonator improved our ability to visualize transplanted cell location non-invasively over a period of 6 weeks., Conclusion: The secondary resonator tuned to enhance the induced B 1 results in improved image uniformity in a pre-clinical application, enabling cell tracking of PFC-labeled cells with the secondary resonator.

Published
2019
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9. Evaluation of the differentiation status of neural stem cells based on cell morphology and the expression of Notch and Sox2.

Author

Ma G, Abbasi F, Koch WT, Mostowski H, Varadkar P, and Mccright B

Subjects
Animals, Biomarkers metabolism, Cells, Cultured, Flow Cytometry, Gene Expression Regulation, Green Fluorescent Proteins genetics, Humans, Mice, Mice, Transgenic, Neural Stem Cells metabolism, Receptor, Notch1 genetics, Receptor, Notch1 metabolism, Receptor, Notch2 genetics, SOXB1 Transcription Factors genetics, Cell Differentiation physiology, Neural Stem Cells cytology, Receptor, Notch2 metabolism, SOXB1 Transcription Factors metabolism
Abstract

Neural stem cells (NSCs) isolated from a variety of sources are being developed as cellular therapies aimed at treating neurodegenerative diseases. During NSC culture and expansion it is important the cells do not differentiate prematurely because this may have an unfavorable effect on product quality and yield. In our study, we evaluated the use of Notch and Sox2 as markers for undifferentiated human and mouse NSCs. The expression of Notch2 and Sox2 during extensive-passage, low-oxygen culture and differentiation conditions were analyzed to confirm that the presence of these signature proteins directly correlates with the ability of NSCs to form new neurospheres and differentiate into multiple cell types. Using expression of Notch1, Notch2 and Sox2 as a reference, we then used flow cytometry to identify a specific morphological profile for undifferentiated murine and human NSCs. Our studies show that Notch and Sox2 expression, along with flow cytometry analysis, can be used to monitor the differentiation status of NSCs grown in culture for use in cellular therapies., (Published by Elsevier Inc.)

Published
2018
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10. Live Cell Imaging of Chromosome Segregation During Mitosis.

Author

Varadkar P, Takeda K, and McCright B

Subjects
Animals, Humans, Mice, Chromosome Segregation genetics, Mitosis genetics, Optical Imaging methods
Abstract

Chromosomes must be reliably and uniformly segregated into daughter cells during mitotic cell division. Fidelity of chromosomal segregation is controlled by multiple mechanisms that include the Spindle Assembly Checkpoint (SAC). The SAC is part of a complex feedback system that is responsible for prevention of a cell progress through mitosis unless all chromosomal kinetochores have attached to spindle microtubules. Chromosomal lagging and abnormal chromosome segregation is an indicator of dysfunctional cell cycle control checkpoints and can be used to measure the genomic stability of dividing cells. Deregulation of the SAC can result in the transformation of a normal cell into a malignant cell through the accumulation of errors during chromosomal segregation. Implementation of the SAC and the formation of the kinetochore complex are tightly regulated by interactions between kinases and phosphatase such as Protein Phosphatase 2A (PP2A). This protocol describes live cell imaging of lagging chromosomes in mouse embryonic fibroblasts isolated from mice that had a knockout of the PP2A-B56γ regulatory subunit. This method overcomes the shortcomings of other cell cycle control imaging techniques such as flow cytometry or immunocytochemistry that only provide a snapshot of a cell cytokinesis status, instead of a dynamic spatiotemporal visualization of chromosomes during mitosis.

Published
2018
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11. RF Safety Evaluation of a Breast Tissue Expander Device for MRI: Numerical Simulation and Experiment.

Author

Park BS, Razjouyan A, Angelone LM, McCright B, and Rajan SS

Abstract

This study describes the MRI-related radio frequency (RF) safety evaluation of breast tissue expander devices to establish safety criteria. Numerical simulations and experimental measurements were performed at 64 MHz with a gel phantom containing a breast expander. Additionally, computational modeling was performed (64 and 128 MHz) with an adult female model, containing a virtually implanted breast tissue expander device for four imaging landmark positions. The presence of the breast tissue expander device led to significant alterations in specific absorption rate (SAR) and|B 1 |distributions. The main source of SAR alterations with the use of the breast expander device was the saline-filled pouch of the expander. Conversely, the variation of RF magnetic field (B + ) was mainly caused by the metallic port. The measured values of electric field magnitude did not increase significantly due to the introduction of the expander device. The maximum 1g- or 10g-averaged SAR values in tissues near the implant were lower than those expected in other regions of the patient body with normalization of both|B 1 + ) was mainly caused by the metallic port. The measured values of electric field magnitude did not increase significantly due to the introduction of the expander device. The maximum 1g- or 10g-averaged SAR values in tissues near the implant were lower than those expected in other regions of the patient body with normalization of both|B 1 + |equal to 2 μ T at the coil isocenter and whole body averaged SAR equal to 4W/kg.

Published
2017
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12. Improvement of Electromagnetic Field Distributions Using High Dielectric Constant (HDC) Materials for CTL-Spine MRI: Numerical Simulations and Experiments.

Author

Park BS, McCright B, Angelone LM, Razjouyan A, and Rajan SS

Abstract

This study investigates the use of pads with high dielectric constant (HDC) materials to alter electromagnetic field distributions in patients during magnetic resonance imaging (MRI). The study was performed with numerical simulations and phantom measurements. An initial proof-of-concept and validation was performed using a phantom at 64 MHz, showing increases of up to 10% in electromagnetic field when using distilled water as the high dielectric material. Additionally, numerical simulations with computational models of human anatomy were performed at 128 MHz. Results of these simulations using barium titanate (BaTiO 3 ) beads showed a 61% increase of [Formula: see text] with a quadrature driven RF coil and a 64% increase with a dual-transmit array. The presence of the HDC material also allowed for a decrease of SAR up to twofold (e.g., peak 10 g-averaged SAR from 54 to 22 W/kg with a quadrature driven RF coil and from 27 to 22 W/kg with a dual-transmit array using CaTiO 3 powder at 128 MHz). The results of this study show that the use of HDC pads at 128 MHz for MRI spine applications could result in improved magnetic fields within the region of interest, while decreasing SAR outside the region.

Published
2017
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13. PP2A-B56γ is required for an efficient spindle assembly checkpoint.

Author

Varadkar P, Abbasi F, Takeda K, Dyson JJ, and McCright B

Subjects
Animals, Apoptosis, Cell Cycle Proteins metabolism, Cells, Cultured, Chromosome Aberrations, Cyclin B1 metabolism, Mice, Knockout, Nocodazole pharmacology, Protein Serine-Threonine Kinases metabolism, Protein Subunits physiology, Protein Transport, M Phase Cell Cycle Checkpoints, Protein Phosphatase 2 physiology
Abstract

The Spindle Assembly Checkpoint (SAC) is part of a complex feedback system designed to ensure that cells do not proceed through mitosis unless all chromosomal kinetochores have attached to spindle microtubules. The formation of the kinetochore complex and the implementation of the SAC are regulated by multiple kinases and phosphatases. BubR1 is a phosphoprotein that is part of the Cdc20 containing mitotic checkpoint complex that inhibits the APC/C so that Cyclin B1 and Securin are not degraded, thus preventing cells going into anaphase. In this study, we found that PP2A in association with its B56γ regulatory subunit, are needed for the stability of BubR1 during nocodazole induced cell cycle arrest. In primary cells that lack B56γ, BubR1 is prematurely degraded and the cells proceed through mitosis. The reduced SAC efficiency results in cells with abnormal chromosomal segregation, a hallmark of transformed cells. Previous studies on PP2A's role in the SAC and kinetochore formation were done using siRNAs to all 5 of the B56 family members. In our study we show that inactivation of only the PP2A-B56γ subunit can affect the efficiency of the SAC. We also provide data that show the intracellular locations of the B56 subunits varies between family members, which is consistent with the hypothesis that they are not completely functionally redundant.

Published
2017
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14. The protein phosphatase 2A B56γ regulatory subunit is required for heart development.

Author

Varadkar P, Despres D, Kraman M, Lozier J, Phadke A, Nagaraju K, and Mccright B

Subjects
Animals, Embryo, Mammalian cytology, Heart Septum cytology, Mice, Mice, Knockout, Mice, Obese, Myocytes, Cardiac cytology, Protein Phosphatase 2 genetics, Embryo, Mammalian enzymology, Heart Septum embryology, Heart Ventricles embryology, Myocytes, Cardiac enzymology, Protein Phosphatase 2 metabolism
Abstract

Background: Protein Phosphatase 2A (PP2A) function is controlled by regulatory subunits that modulate the activity of the catalytic subunit and direct the PP2A complex to specific intracellular locations. To study PP2A's role in signal transduction pathways that control growth and differentiation in vivo, a transgenic mouse lacking the B56γ regulatory subunit of PP2A was made., Results: Lack of PP2A activity specific to the PP2A-B56γ holoenzyme, resulted in the formation of an incomplete ventricular septum and a decrease in the number of ventricular cardiomyocytes. During cardiac development, B56γ is expressed in the nucleus of α-actinin-positive cardiomyocytes that contain Z-bands. The pattern of B56γ expression correlated with the cardiomyocyte apoptosis we observed in B56γ-deficient mice during mid to late gestation. In addition to the cardiac phenotypes, mice lacking B56γ have a decrease in locomotive coordination and gripping strength, indicating that B56γ has a role in controlling PP2A activity required for efficient neuromuscular function., Conclusions: PP2A-B56γ activity is required for efficient cardiomyocyte maturation and survival. The PP2A B56γ regulatory subunit controls PP2A substrate specificity in vivo in a manner that cannot be fully compensated for by other B56 subunits., (© 2014 Wiley Periodicals, Inc.)

Published
2014
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15. A disintegrin and metalloproteinase 10 regulates antibody production and maintenance of lymphoid architecture.

Author

Chaimowitz NS, Martin RK, Cichy J, Gibb DR, Patil P, Kang DJ, Farnsworth J, Butcher EC, McCright B, and Conrad DH

Subjects
ADAM Proteins biosynthesis, ADAM Proteins deficiency, ADAM10 Protein, Amyloid Precursor Protein Secretases biosynthesis, Amyloid Precursor Protein Secretases deficiency, Animals, B-Lymphocyte Subsets enzymology, B-Lymphocyte Subsets immunology, B-Lymphocyte Subsets pathology, CHO Cells, Cricetinae, Germinal Center enzymology, Germinal Center immunology, Germinal Center pathology, Lymphocyte Activation genetics, Lymphocyte Activation immunology, Membrane Proteins biosynthesis, Membrane Proteins deficiency, Mice, Mice, Inbred BALB C, Mice, Knockout, Mice, Transgenic, Peyer's Patches enzymology, Peyer's Patches immunology, Peyer's Patches pathology, T-Lymphocyte Subsets cytology, T-Lymphocyte Subsets enzymology, T-Lymphocyte Subsets immunology, Up-Regulation genetics, Up-Regulation immunology, ADAM Proteins physiology, Amyloid Precursor Protein Secretases physiology, Immunity, Humoral genetics, Membrane Proteins physiology
Abstract

A disintegrin and metalloproteinase 10 (ADAM10) is a zinc-dependent proteinase related to matrix metalloproteinases. ADAM10 has emerged as a key regulator of cellular processes by cleaving and shedding extracellular domains of multiple transmembrane receptors and ligands. We have developed B cell-specific ADAM10-deficient mice (ADAM10(B-/-)). In this study, we show that ADAM10 levels are significantly enhanced on germinal center B cells. Moreover, ADAM10(B-/-) mice had severely diminished primary and secondary responses after T-dependent immunization. ADAM10(B-/-) displayed impaired germinal center formation, had fewer follicular Th cells, decreased follicular dendritic cell networks, and altered chemokine expression in draining lymph nodes (LNs). Interestingly, when spleen and LN structures from immunized mice were analyzed for B and T cell localization, tissues structure was aberrant in ADAM10(B-/-) mice. Importantly, when ADAM10-deficient B cells were stimulated in vitro, they produced comparable Ab as wild type B cells. This result demonstrates that the defects in humoral responses in vivo result from inadequate B cell activation, likely because of the decrease in follicular Th cells and the changes in structure. Thus, ADAM10 is essential for the maintenance of lymphoid structure after Ag challenge.

Published
2011
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16. The contribution of Notch1 to nephron segmentation in the developing kidney is revealed in a sensitized Notch2 background and can be augmented by reducing Mint dosage.

Author

Surendran K, Boyle S, Barak H, Kim M, Stomberski C, McCright B, and Kopan R

Subjects
Animals, Cell Survival, Epithelial Cells cytology, Epithelial Cells metabolism, Green Fluorescent Proteins metabolism, Homeodomain Proteins metabolism, Immunoglobulin J Recombination Signal Sequence-Binding Protein metabolism, Integrases metabolism, Kidney Glomerulus cytology, Kidney Glomerulus metabolism, Kidney Tubules, Proximal cytology, Kidney Tubules, Proximal metabolism, Mesoderm cytology, Mesoderm metabolism, Mice, Mosaicism, PAX3 Transcription Factor, Paired Box Transcription Factors metabolism, Receptor, Notch2 metabolism, Repressor Proteins metabolism, Stem Cells cytology, Stem Cells metabolism, Transcription Factors metabolism, Transcription, Genetic, Transgenes genetics, Adaptor Proteins, Signal Transducing metabolism, Gene Dosage genetics, Nephrons embryology, Nephrons metabolism, Nerve Tissue Proteins metabolism, Receptor, Notch1 metabolism
Abstract

We previously determined that Notch2, and not Notch1, was required for forming proximal nephron segments. The dominance of Notch2 may be conserved in humans, since Notch2 mutations occur in Alagille syndrome (ALGS) 2 patients, which includes renal complications. To test whether mutations in Notch1 could increase the severity of renal complications in ALGS, we inactivated conditional Notch1 and Notch2 alleles in mice using a Six2-GFP::Cre. This BAC transgene is expressed mosaically in renal epithelial progenitors but uniformly in cells exiting the progenitor pool to undergo mesenchymal-to-epithelial transition. Although delaying Notch2 inactivation had a marginal effect on nephron numbers, it created a sensitized background in which the inactivation of Notch1 severely compromised nephron formation, function, and survival. These and additional observations indicate that Notch1 in concert with Notch2 contributes to the morphogenesis of renal vesicles into S-shaped bodies in a RBP-J-dependent manner. A significant implication is that elevating Notch1 activity could improve renal functions in ALGS2 patients. As proof of principle, we determined that conditional inactivation of Mint, an inhibitor of Notch-RBP-J interaction, resulted in a moderate rescue of Notch2 null kidneys, implying that temporal blockage of Notch signaling inhibitors downstream of receptor activation may have therapeutic benefits for ALGS patients., (Copyright 2009 Elsevier Inc. All rights reserved.)

Published
2010
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17. Generation of mice that conditionally express the activation domain of Notch2.

Author

Varadkar PA, Kraman M, and McCright B

Subjects
Animals, Base Sequence, Cell Proliferation, DNA Primers, Female, Immunohistochemistry, In Situ Nick-End Labeling, Mice, Mice, Transgenic, Pregnancy, Receptor, Notch2 genetics
Abstract

The Notch pathway is an intercellular signaling mechanism frequently used for controlling cell fate during organogenesis. There are four structurally related Notch receptors in mice and humans, and Notch1 and Notch2 are essential genes. In this report we describe the construction of a transgenic mouse strain that expresses the Notch2 intracellular domain in response to cell lineage specific expression of Cre recombinase. This approach bypasses the requirement for ligand- receptor interaction and allows the direct determination of the consequences of Notch2 activation in vivo. Exogenous expression of the Notch2 intracellular domain resulted in the developmental arrest of secondary heart field derived cardiomyocytes during the transition from immature alpha-Smooth Muscle Actin expressing cells to mature alpha-Actinin positive cardiomyocytes. In contrast, a cell nonautonomous mesenchymal expansion was observed in semilunar valves. This new conditionally expressed allele of Notch2 can be used in studies by investigators interested in the effects of Notch2 activation in vivo.

Published
2009
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19. Notch2 is required for the proliferation of cardiac neural crest-derived smooth muscle cells.

Author

Varadkar P, Kraman M, Despres D, Ma G, Lozier J, and McCright B

Subjects
Actins metabolism, Animals, Arteries anatomy & histology, Arteries diagnostic imaging, Arteries metabolism, Cell Lineage, Cell Movement physiology, Female, Genes, Reporter, Genotype, Humans, Mice, Mice, Inbred C57BL, Myocytes, Smooth Muscle cytology, Phenotype, Receptor, Notch2 genetics, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Ultrasonography, Cell Proliferation, Heart anatomy & histology, Heart embryology, Myocytes, Smooth Muscle physiology, Neural Crest cytology, Receptor, Notch2 metabolism
Abstract

Mutations in Notch receptors and their ligands have been identified as the cause of human congenital heart diseases, indicating the importance of the Notch signaling pathway during heart development. In our study, we use Cre-Lox technology to inactivate Notch2 in several cardiac cell lineages to determine the functional requirements for Notch2 during mammalian heart development. Inactivation of Notch2 in cardiac neural crest cells resulted in abnormally narrow aortas and pulmonary arteries due to a decrease in smooth muscle tissue. The reduction in smooth muscle tissue was not due to cell migration defects but instead was found to be caused by less proliferation in smooth muscle cells during mid to late gestation. Our findings demonstrate that Notch2 is required cell autonomously for proper formation of the heart outflow tract and provides insights into the role of Notch2 in vascular smooth muscle development and the cardiovascular defects associated with Alagille syndrome., ((c) 2008 Wiley-Liss, Inc.)

Published
2008
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20. Notch signaling regulates bile duct morphogenesis in mice.

Author

Lozier J, McCright B, and Gridley T

Subjects
Animals, Heterozygote, Immunohistochemistry, Mice, Receptors, Notch genetics, Bile Ducts growth & development, Morphogenesis, Receptors, Notch metabolism, Signal Transduction
Abstract

Background: Alagille syndrome is a developmental disorder caused predominantly by mutations in the Jagged1 (JAG1) gene, which encodes a ligand for Notch family receptors. A characteristic feature of Alagille syndrome is intrahepatic bile duct paucity. We described previously that mice doubly heterozygous for Jag1 and Notch2 mutations are an excellent model for Alagille syndrome. However, our previous study did not establish whether bile duct paucity in Jag1/Notch2 double heterozygous mice resulted from impaired differentiation of bile duct precursor cells, or from defects in bile duct morphogenesis., Methodology/principal Findings: Here we characterize embryonic biliary tract formation in our previously described Jag1/Notch2 double heterozygous Alagille syndrome model, and describe another mouse model of bile duct paucity resulting from liver-specific deletion of the Notch2 gene., Conclusions/significance: Our data support a model in which bile duct paucity in Notch pathway loss of function mutant mice results from defects in bile duct morphogenesis rather than cell fate specification.

Published
2008
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21. Direct regulation of Gata3 expression determines the T helper differentiation potential of Notch.

Author

Amsen D, Antov A, Jankovic D, Sher A, Radtke F, Souabni A, Busslinger M, McCright B, Gridley T, and Flavell RA

Subjects
Animals, Base Sequence, Cells, Cultured, GATA3 Transcription Factor biosynthesis, GATA3 Transcription Factor physiology, Humans, Immunoglobulin J Recombination Signal Sequence-Binding Protein deficiency, Immunoglobulin J Recombination Signal Sequence-Binding Protein genetics, Immunoglobulin J Recombination Signal Sequence-Binding Protein physiology, Mice, Mice, Inbred C57BL, Mice, Knockout, Mice, Transgenic, Molecular Sequence Data, Signal Transduction immunology, T-Lymphocytes, Helper-Inducer metabolism, Th1 Cells cytology, Th1 Cells immunology, Th1 Cells metabolism, Th2 Cells cytology, Th2 Cells immunology, Th2 Cells metabolism, Cell Differentiation immunology, GATA3 Transcription Factor metabolism, Receptors, Notch physiology, T-Lymphocytes, Helper-Inducer cytology, T-Lymphocytes, Helper-Inducer immunology
Abstract

CD4(+) T helper cells differentiate into T helper 1 (Th1) or Th2 effector lineages, which orchestrate immunity to different types of microbes. Both Th1 and Th2 differentiation can be induced by Notch, but what dictates which of these programs is activated in response to Notch is not known. By using T cell-specific gene ablation of the Notch effector RBP-J or the Notch1 and 2 receptors, we showed here that Notch was required on CD4(+) T cells for physiological Th2 responses to parasite antigens. GATA-3 was necessary for Notch-induced Th2 differentiation, and we identified an upstream Gata3 promoter as a direct target for Notch signaling. Moreover, absence of GATA-3 turned Notch from a Th2 inducer into a powerful inducer of Th1 differentiation. Therefore, Gata3 is a critical element determining inductive Th2 differentiation and limiting Th1 differentiation by Notch.

Published
2007
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22. Generation of new Notch2 mutant alleles.

Author

McCright B, Lozier J, and Gridley T

Subjects
Animals, Base Sequence, Blotting, Northern, DNA Primers, Mice, Mice, Inbred C57BL, Mice, Knockout, Reverse Transcriptase Polymerase Chain Reaction, Alleles, Mutation, Receptor, Notch2 genetics
Abstract

The Notch signaling pathway is an evolutionarily conserved intercellular signaling mechanism, and mutations in its components disrupt embryonic development in many organisms and cause inherited diseases in humans. We previously described construction and analysis of a hypomorphic allele of the Notch2 gene. Homozygosity for this allele leads to embryonic and perinatal lethality due to cardiovascular and kidney defects. We report here novel Notch2 mutant alleles generated by gene targeting in embryonic stem cells, including a conditional null allele in which exon 3 of the Notch2 gene is flanked by loxP sequences. These new Notch2 mutant alleles expand the set of tools available for studying the myriad roles of the Notch pathway during mammalian development and will enable analysis of Notch2 function at additional stages of embryogenesis and in adult mice., ((c) 2006 Wiley-Liss, Inc.)

Published
2006
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23. Functional conservation of Notch1 and Notch2 intracellular domains.

Author

Kraman M and McCright B

Subjects
Alleles, Animals, Conserved Sequence, Female, Mice, Mice, Inbred C57BL, Mice, Inbred ICR, Phenotype, Protein Structure, Tertiary, RNA, Messenger analysis, Receptor, Notch1 chemistry, Receptor, Notch1 genetics, Receptor, Notch2 chemistry, Receptor, Notch2 genetics, Recombinant Proteins biosynthesis, Recombinant Proteins genetics, Receptor, Notch1 physiology, Receptor, Notch2 physiology
Abstract

The Notch receptor is a key component of a highly conserved signaling pathway that regulates cell fate determination during development. In Drosophila, where Notch signaling was first identified and studied, there is only one Notch receptor. In contrast, mammals have four Notch receptor genes, Notch1-4. Notch1 and Notch2 are both required for embryo viability, are widely expressed in mammals, and are structurally conserved. It is presently unknown if these two receptors are functionally redundant or if they have unique capabilities related to differences in their amino acid sequences. In contrast to the rest of the molecule, the amino acid sequences of a large region of the Notch intracellular domain are not highly conserved and thus may be able to interact with distinct transcription factors and mediate the expression of different sets of genes. To determine if the function of this region is conserved, the last 426 amino acids of the Notch2 receptor have been replaced with the corresponding region of Notch1 in mice by using gene targeting. We have determined that even though the amino acid sequences of this region are only 37% identical (137/426), the C-terminal region of the Notch1 intracellular domain can functionally replace that of Notch2 in vivo.

Published
2005
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24. Notch signaling in kidney development.

Author

McCright B

Subjects
Animals, Calcium-Binding Proteins, Humans, Intercellular Signaling Peptides and Proteins, Jagged-1 Protein, Kidney physiology, Membrane Proteins, Mice, Mutation, Proteins physiology, Receptor, Notch2, Renal Circulation physiology, Serrate-Jagged Proteins, Kidney growth & development, Receptors, Cell Surface physiology, Signal Transduction physiology
Abstract

Purpose of Review: Notch signaling is a highly conserved mechanism used by multicellular animals to specify cell fate decisions during the formation of complex structures such as the kidney. A number of studies have recently identified requirements for Notch signaling during kidney organogenesis and tissue repair. This review will summarize these studies and compare Notch signaling in the mammalian kidney with Notch signaling in other organ systems., Recent Findings: A targeted mutation in the mouse Notch2 receptor resulted in kidneys that are devoid of glomerular endothelial and mesangial cells. The mutant epithelial cells of the developing glomerulus have reduced amounts of vascular endothelial growth factor expression, which may be responsible for the lack of vascularization observed in these glomeruli. Notch2 is expressed in the epithelial cells of the developing glomerulus, and a potential ligand, Jagged1 is expressed in the endothelial cells of the glomerulus. Mice simultaneously heterozygous for mutations in both Notch2 and Jagged1 phenocopy the kidney defects seen in mice homozygous for the Notch2 mutation. These doubly heterozygous mice also display liver and heart developmental abnormalities reminiscent of Alagille's syndrome., Summary: Notch signaling is required for kidney development, and the expression of Notch genes is increased in response to kidney damage. Further studies of Notch signaling will be important in order to understand kidney development and tissue repair.

Published
2003
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25. A mouse model of Alagille syndrome: Notch2 as a genetic modifier of Jag1 haploinsufficiency.

Author

McCright B, Lozier J, and Gridley T

Subjects
Alagille Syndrome etiology, Animals, Bile Ducts embryology, Bile Ducts pathology, Calcium-Binding Proteins, Cell Differentiation, Disease Models, Animal, Drosophila Proteins, Heart embryology, Heart Defects, Congenital etiology, Heart Defects, Congenital genetics, Heart Defects, Congenital pathology, Intercellular Signaling Peptides and Proteins, Jagged-1 Protein, Liver embryology, Membrane Proteins, Mice, Mice, Inbred C57BL, Mutagenesis, Phenotype, Receptor, Notch2, Serrate-Jagged Proteins, Alagille Syndrome genetics, Proteins genetics, Receptors, Cell Surface genetics
Abstract

Alagille syndrome is a human autosomal dominant developmental disorder characterized by liver, heart, eye, skeletal, craniofacial and kidney abnormalities. Alagille syndrome is caused by mutations in the Jagged 1 (JAG1) gene, which encodes a ligand for Notch family receptors. The majority of JAG1 mutations seen in Alagille syndrome patients are null alleles, suggesting JAG1 haploinsufficiency as a primary cause of this disorder. Mice homozygous for a Jag1 null mutation die during embryogenesis and Jag1/+ heterozygous mice exhibit eye defects but do not exhibit other phenotypes characteristic of Alagille syndrome patients ( Xue, Y., Gao, X., Lindsell, C. E., Norton, C. R., Chang, B., Hicks, C., Gendron-Maguire, M., Rand, E. B., Weinmaster, G. and Gridley, T. (1999) HUM: Mol. Genet. 8, 723-730). Here we report that mice doubly heterozygous for the Jag1 null allele and a Notch2 hypomorphic allele exhibit developmental abnormalities characteristic of Alagille syndrome. Double heterozygous mice exhibit jaundice, growth retardation, impaired differentiation of intrahepatic bile ducts and defects in heart, eye and kidney development. The defects in bile duct epithelial cell differentiation and morphogenesis in the double heterozygous mice are similar to defects in epithelial morphogenesis of Notch pathway mutants in Drosophila, suggesting that a role for the Notch signaling pathway in regulating epithelial morphogenesis has been conserved between insects and mammals. This work also demonstrates that the Notch2 and Jag1 mutations interact to create a more representative mouse model of Alagille syndrome and provides a possible explanation of the variable phenotypic expression observed in Alagille syndrome patients.

Published
2002
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27. The B56 family of protein phosphatase 2A (PP2A) regulatory subunits encodes differentiation-induced phosphoproteins that target PP2A to both nucleus and cytoplasm.

Author

McCright B, Rivers AM, Audlin S, and Virshup DM

Subjects
Adult, Base Sequence, Biological Transport, Active, Cloning, Molecular, Humans, Isoenzymes biosynthesis, Molecular Sequence Data, Phosphoprotein Phosphatases metabolism, Phosphorylation, Protein Conformation, Protein Phosphatase 2, Sequence Homology, Nucleic Acid, Software, Structure-Activity Relationship, Tretinoin pharmacology, Up-Regulation drug effects, Cell Nucleus metabolism, Cytoplasm metabolism, Phosphoprotein Phosphatases genetics, Phosphoproteins biosynthesis
Abstract

Protein phosphatase 2A is a heterotrimeric protein serine/threonine phosphatase consisting of a 36-kDa catalytic C subunit, a 65-kDa structural A subunit, and a variable regulatory B subunit. The B subunits determine the substrate specificity of the enzyme. There have been three families of cellular B subunits identified to date: B55, B56 (B'), and PR72/130. We have now cloned five genes encoding human B56 isoforms. Polypeptides encoded by all but one splice variant (B56gamma1) are phosphoproteins, as shown by mobility shift after treatment with alkaline phosphatase and metabolic labeling with [32P]phosphate. All labeled isoforms contain solely phosphoserine. Indirect immunofluorescence microscopy demonstrates distinct patterns of intracellular targeting by different B56 isoforms. Specifically, B56alpha, B56beta, and B56epsilon complexed with the protein phosphatase 2A A and C subunits localize to the cytoplasm, whereas B56delta, B56gamma1, and B56gamma3 are concentrated in the nucleus. Two isoforms (B56beta and B56delta) are highly expressed in adult brain; here we show that mRNA for these isoforms increases severalfold when neuroblastoma cell lines are induced to differentiate by retinoic acid treatment. These studies demonstrate an increasing diversity of regulatory mechanisms to control the activity of this key intracellular protein phosphatase and suggest distinct functions for isoforms targeted to different intracellular locations.

Published
1996
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28. Assignment of human protein phosphatase 2A regulatory subunit genes b56alpha, b56beta, b56gamma, b56delta, and b56epsilon (PPP2R5A-PPP2R5E), highly expressed in muscle and brain, to chromosome regions 1q41, 11q12, 3p21, 6p21.1, and 7p11.2 --> p12.

Author

McCright B, Brothman AR, and Virshup DM

Subjects
Brain Chemistry, Chromosomes, Human genetics, Humans, In Situ Hybridization, Fluorescence, Isoenzymes genetics, Muscle, Skeletal chemistry, Myocardium chemistry, Organ Specificity, Protein Phosphatase 2, RNA, Messenger analysis, Chromosome Mapping, Gene Expression Regulation, Enzymologic, Phosphoprotein Phosphatases genetics
Abstract

The activity of the major intracellular protein phosphatase, protein phosphatase 2A (PP2A), is determined by the nature of the associated regulatory subunit. A new family of human PP2A regulatory subunits has recently been identified. Three of these subunits, B56beta, B56delta, and B56epsilon, are most highly expressed in brain, while the B56alpha and B56gamma isoforms are highly expressed in cardiac and skeletal muscle. Genes PPP2R5A-PPP2R5E encoding the phosphatase regulatory proteins B56alpha, B56beta, B56gamma, B56delta, and B56epsilon have now been mapped by fluorescence in situ hybridization to chromosome regions 1q41, 11q12, 3p21, 6p21.1, and 7p11.2 --> p12, respectively.

Published
1996
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