Your search keyword '"Heng-Phon Too"' showing total 34 results

1. A highly efficient non-viral process for programming mesenchymal stem cells for gene directed enzyme prodrug cancer therapy

Author

Jun Yung Woo, Yoon Khei Ho, Geraldine Xue En Tu, Lih-Wen Deng, and Heng-Phon Too

Subjects

0301 basic medicine, Adolescent, Genetic Vectors, lcsh:Medicine, Mice, Nude, Mesenchymal Stem Cell Transplantation, Transfection, Article, Viral vector, Viral process, 03 medical and health sciences, Mice, Young Adult, 0302 clinical medicine, Cell Line, Tumor, Neoplasms, Animals, Humans, Polyethyleneimine, Prodrugs, Gene delivery, lcsh:Science, Cancer, Multidisciplinary, Chemistry, lcsh:R, Mesenchymal stem cell, Cytosine deaminase, Mesenchymal Stem Cells, Genetic Therapy, Prodrug, 030104 developmental biology, Cell culture, Cancer cell, Genetic engineering, Cancer research, lcsh:Q, Female, Glioblastoma, 030217 neurology & neurosurgery

Abstract

Mesenchymal stem cells (MSCs) driven gene-directed enzyme prodrug therapy has emerged as a potential strategy for cancer treatment. The tumour-nesting properties of MSCs enable these vehicles to target tumours and metastases with effective therapies. A crucial step in engineering MSCs is the delivery of genetic material with low toxicity and high efficiency. Due to the low efficiency of current transfection methods, viral vectors are used widely to modify MSCs in preclinical and clinical studies. We show, for the first time, the high transfection efficiency (> 80%) of human adipose tissue derived-MSCs (AT-MSCs) using a cost-effective and off-the-shelf Polyethylenimine, in the presence of histone deacetylase 6 inhibitor and fusogenic lipids. Notably, the phenotypes of MSCs remained unchanged post-modification. AT-MSCs engineered with a fused transgene, yeast cytosine deaminase::uracil phosphoribosyltransferase (CDy::UPRT) displayed potent cytotoxic effects against breast, glioma, gastric cancer cells in vitro. The efficiency of eliminating gastric cell lines were effective even when using 7-day post-transfected AT-MSCs, indicative of the sustained expression and function of the therapeutic gene. In addition, significant inhibition of temozolomide resistant glioma tumour growth in vivo was observed with a single dose of therapeutic MSC. This study demonstrated an efficient non-viral modification process for MSC-based prodrug therapy.

Published

2020

2. Nano-topology guided neurite outgrowth in PC12 cells is mediated by miRNAs

Author

Lihan Zhou, He Cheng, Mei Zhu, Heng-Phon Too, Wee Kiong Choi, and Bihan Li

Subjects

Neurite, Polyethylene Terephthalates, Cell model, technology, industry, and agriculture, Biomedical Engineering, Pharmaceutical Science, Medicine (miscellaneous), Bioengineering, Biology, Topology, PC12 Cells, Rats, MicroRNAs, microRNA, Gene expression, Neurites, Animals, Humans, Molecular Medicine, General Materials Science, Intracellular

Abstract

MicroRNAs (miRNAs) are master regulators of gene expression at post-transcriptional level. The present study investigated the involvement of miRNAs in topological guidance of neurite outgrowth in an NGF treated PC12 cell model cultured on nano-patterned polyethylene terephthalate (PET) substrates fabricated with interference lithography. The expressions of 38 neuronal miRNAs were measured and 3 were found to be differentially regulated during topological guidance of neurite outgrowth. Altering the intracellular levels of these miRNAs disrupted the orderly growth of neurite along nano-patterned substrate. Our results showed miRNAs to be versatile regulators and their involvement should be thoroughly investigated for better understanding of biological processes. From the Clinical Editor In this basic science study, strong evidence was found that topological guidance is only one factor, and miRNA-s regulate axonal outgrowth from neurites. Nano-patterned polyethylene terephthalate substrates were used for the study, fabricated using interference lithography. Further studies of this biologically relevant process may pave the way to clinically useful axonal regrowth and axonal guidance methods.

Published

2014

3. High-frequency stimulation of the globus pallidus interna nucleus modulates GFRα1 gene expression in the basal ganglia

Author

Heng-Phon Too, Jiayi Tan, Yong Chee Tan, Duncun Xun Kiat Ho, and Wai Hoe Ng

Subjects

Male, Nervous system, medicine.medical_specialty, Glial Cell Line-Derived Neurotrophic Factor Receptors, Deep brain stimulation, Deep Brain Stimulation, medicine.medical_treatment, Gene Expression, Stimulation, Globus Pallidus, Neuroprotection, Basal Ganglia, Physiology (medical), Internal medicine, Basal ganglia, RNA Isoforms, medicine, Glial cell line-derived neurotrophic factor, Animals, RNA, Messenger, Rats, Wistar, biology, business.industry, Dopaminergic, General Medicine, Rats, Alternative Splicing, Endocrinology, Globus pallidus, medicine.anatomical_structure, nervous system, Neurology, biology.protein, Surgery, Neurology (clinical), business

Abstract

Deep brain stimulation (DBS) is an established therapy for movement disorders such as Parkinson's disease (PD). Although the efficacy of DBS is clear, its precise molecular mechanism remains unknown. The glial cell line derived factor (GDNF) family of ligands has been shown to confer neuroprotective effects on dopaminergic neurons, and putaminal infusion of GDNF have been investigated in PD patients with promising results. Despite the potential therapeutic role of GDNF in alleviating motor symptoms, there is no data on the effects of electrical stimulation on GDNF-family receptor (GFR) expression in the basal ganglia structures. Here, we report the effects of electrical stimulation on GFRα1 isoforms, particularly GFRα1a and GFRα1b. Wistar rats underwent 2 hours of high frequency stimulation (HFS) at the globus pallidus interna nucleus. A control group was subjected to a similar procedure but without stimulation. The HFS group, sacrificed 24 hours after treatment, had a threefold decrease in mRNA expression level of GFRα1b (p=0.037), but the expression level reverted to normal 72 hours after stimulation. Our preliminary data reveal the acute effects of HFS on splice isoforms of GFRα1, and suggest that HFS may modulate the splice isoforms of GFRα1a and GFRα1b to varying degrees. Going forward, elucidating the interactions between HFS and GFR may shed new insights into the complexity of GDNF signaling in the nervous system and lead to better design of clinical trials using these signaling pathways to halt disease progression in PD and other neurodegenerative diseases.

Published

2014

4. GDNF family ligand dependent STAT3 activation is mediated by specific alternatively spliced isoforms of GFRα2 and RET

Author

Heng-Phon Too and Lihan Zhou

Subjects

STAT3 Transcription Factor, Glial Cell Line-Derived Neurotrophic Factor Receptors, Neurite, Neurturin, Ligands, PC12 Cells, Receptor isoform, Mice, Phosphoserine, Neurites, Glial cell line-derived neurotrophic factor, Animals, Protein Isoforms, Phosphorylation, Tyrosine, Extracellular Signal-Regulated MAP Kinases, STAT3, Neural Cell Adhesion Molecules, Molecular Biology, Cell Nucleus, biology, Proto-Oncogene Proteins c-ret, Mitochondrial STAT3, Cell Biology, GDNF, Mitochondria, Rats, Alternative Splicing, Protein Transport, NRTN, src-Family Kinases, GFRα2, biology.protein, Cancer research, Neural cell adhesion molecule, RET, GDNF family of ligands

Abstract

Neurturin (NRTN), a member of the GDNF family of ligands (GFL), is currently investigated in a series of clinical trials for Parkinson's disease. NRTN signals through its cognate receptor GFRα2 and co-receptor RET to induce neurite outgrowth, but the underlying mechanism remains to be better understood. STAT3 was previously shown to be activated by oncogenic RET, independent of ligand and GFRα. In this study, we demonstrated that NRTN induced serine727 but not tyrosine705 phosphorylation of STAT3 in primary cortical neuron and neuronal cell lines. Remarkably, STAT3 phosphorylation was found to be mediated specifically by GFRα2c and RET9 isoforms. Furthermore, serine but not tyrosine dominant negative mutant of STAT3 impaired NRTN induced neurite outgrowth, indicative of the role of STAT3 as a downstream mediator of NRTN function. Similar to NGF, the NRTN induced P-Ser-STAT3 was localized to the mitochondria but not to the nucleus. Mitochondrial STAT3 was further found to be intimately involved in NRTN induced neurite outgrowth. Collectively, these findings demonstrated the hitherto unrecognized and novel role of specific GFRα2 and RET isoforms in mediating NRTN activation of STAT3 and the transcription independent mechanism whereby the mitochondria localized P-Ser-STAT3 mediated NRTN induced neurite outgrowth.

Published

2013

5. Spatially resolved microrheology of heterogeneous biopolymer hydrogels using covalently bound microspheres

Author

LH Long Wong, H-P Heng-Phon Too, Nicholas A. Kurniawan, Raj Rajagopalan, and Soft Tissue Biomech. & Tissue Eng.

Subjects

Microrheology, Biopolymer, Microenvironment, Materials science, Surface Properties, Green Fluorescent Proteins, Acrylic Resins, Nanotechnology, engineering.material, Biopolymers, Rheology, Materials Testing, Animals, Particle Size, Elasticity (economics), Serum Albumin, Microscopy, Confocal, Viscosity, Mechanical Engineering, Hydrogels, Glioma, Carbon, Elasticity, Microspheres, Extracellular Matrix, Rats, Particle-tracking, Modeling and Simulation, Self-healing hydrogels, engineering, Surface modification, Cattle, Collagen, Stress, Mechanical, Particle size, Heterogeneous network, Biotechnology

Abstract

Characterization of the rheological properties of heterogeneous biopolymers is important not only to understand the effect of substrate elasticity on cell behaviors, but also to provide insights into mechanical changes during cellular remodeling of the environment. Conventional particle-tracking microrheology (PTM) techniques are compromised by probe–network slippage and cage-hopping problems, and require a priori knowledge of network mesh size in order to determine a suitable probe size. We demonstrated here the usefulness of covalently bound probes for PTM of biopolymers to overcome the above limitations. We showed that, in a well-defined system like polyacrylamide gels, surface-modified probe particles using a zero-length crosslinker provided more reliable measurements of network mechanics as compared to standard carboxylated probes. We further demonstrated that appropriate surface modification of microspheres for PTM circumvented the requirement of using microspheres larger than the network mesh, an approach typically considered to be ideal. Using the method presented in this study, we found the local network at the leading edge of a typical C6 glioma cell to be stiffer as compared to the side. Our findings established that permanent interaction between the probe and network is crucial to reliably measure the local network mechanics in reconstituted, heterogeneous networks using PTM.

Published

2013

6. Enhanced non-viral gene delivery by coordinated endosomal release and inhibition of β-tubulin deactylase

Author

Li Han Zhou, Yoon Khei Ho, Kam Chiu Tam, and Heng-Phon Too

Subjects

0301 basic medicine, Indoles, Polymers, Cellular differentiation, viruses, Endosomes, Biology, Gene delivery, Hydroxamic Acids, Transfection, Cell Line, Small hairpin RNA, 03 medical and health sciences, Mice, 0302 clinical medicine, Neural Stem Cells, Tubulin, Genetics, Animals, Cells, Cultured, Mesenchymal stem cell, fungi, Acetylation, Biological Transport, Cell Differentiation, DNA, Hydrogen-Ion Concentration, Neural stem cell, Cell biology, Histone Deacetylase Inhibitors, 030104 developmental biology, Cell culture, 030220 oncology & carcinogenesis, Methods Online, Stem cell

Abstract

Efficient non-viral gene delivery is highly desirable but often unattainable with some cell-types. We report here that non-viral DNA polyplexes can efficiently transfect differentiated neuronal and stem cells. Polyplex transfection centrifugation protocols was enhanced by including a simultaneous treatment with a DOPE/CHEMS lipid suspension and a microtubule inhibitor, Tubastatin A. Lipoplex transfection protocols were not improved by this treatment. This mechanism of action was unravelled by systematically identifying and rationally mitigating barriers limiting high transfection efficiency, allowing unexpected improvements in the transfection of mesenchymal stem cells (MSC), primary neuron and several hard-to-transfect cell types beyond what are currently achievable using cationic polymers. The optimized formulation and method achieved high transfection efficiency with no adverse effects on cell viability, cell proliferation or differentiation. High efficiency modification of MSC for cytokine overexpression, efficient generation of dopaminergic neuron using neural stem cells and enhanced genome editing with CRISPR-Cas9 were demonstrated. In summary, this study described a cost-effective method for efficient, rapid and scalable workflow for ex vivo gene delivery using a myriad of nucleic acids including plasmid DNA, mRNA, siRNA and shRNA.

Published

2016

7. snoU6 and 5S RNAs are not reliable miRNA reference genes in neuronal differentiation

Author

Heng-Phon Too, Qing-En Lim, Yoon Khei Ho, Guoqiang Wan, and Lihan Zhou

Subjects

Cell type, RNA Stability, Neuronal differentiation, Computational biology, Biology, Real-Time Polymerase Chain Reaction, Cell Line, Transcriptome, Mice, RNA, Small Nuclear, Reference genes, microRNA, Gene expression, Animals, Humans, Neurons, Genetics, Reverse Transcriptase Polymerase Chain Reaction, Gene Expression Profiling, General Neuroscience, RNA, Ribosomal, 5S, RNA, Cell Differentiation, Reference Standards, Ribosomal RNA, Immunohistochemistry, Rats, MicroRNAs

Abstract

Accurate profiling of microRNAs (miRNAs) is an essential step for understanding the functional significance of these small RNAs in both physiological and pathological processes. Quantitative real-time PCR (qPCR) has gained acceptance as a robust and reliable transcriptomic method to profile subtle changes in miRNA levels and requires reference genes for accurate normalization of gene expression. 5S and snoU6 RNAs are commonly used as reference genes in microRNA quantification. It is currently unknown if these small RNAs are stably expressed during neuronal differentiation. Panels of miRNAs have been suggested as alternative reference genes to 5S and snoU6 in various physiological contexts. To test the hypothesis that miRNAs may serve as stable references during neuronal differentiation, the expressions of eight miRNAs, 5S and snoU6 RNAs in five differentiating neuronal cell types were analyzed using qPCR. The stabilities of the expressions were evaluated using two complementary statistical approaches (geNorm and Normfinder). Expressions of 5S and snoU6 RNAs were stable under some but not all conditions of neuronal differentiation and thus are not suitable reference genes. In contrast, a combination of three miRNAs (miR-103, miR-106b and miR-26b) allowed accurate expression normalization across different models of neuronal differentiation.

Published

2011

8. GDNF-induced cell signaling and neurite outgrowths are differentially mediated by GFRalpha1 isoforms

Author

Guoqiang Wan, Heng-Phon Too, and Li Foong Yoong

Subjects

Central Nervous System, rac1 GTP-Binding Protein, Cell signaling, Glial Cell Line-Derived Neurotrophic Factor Receptors, RHOA, Neurite, Biology, Transfection, Mice, Neuroblastoma, Cellular and Molecular Neuroscience, Neurotrophic factors, Cell Line, Tumor, Neurites, Glial cell line-derived neurotrophic factor, Animals, Humans, Protein Isoforms, Glial Cell Line-Derived Neurotrophic Factor, cdc42 GTP-Binding Protein, Molecular Biology, Neurturin, Cell Differentiation, Cell Biology, Molecular biology, Rho Factor, Cell biology, DNA-Binding Proteins, nervous system, Cdc42 GTP-Binding Protein, biology.protein, Neural cell adhesion molecule, GDNF family of ligands, Signal Transduction, Transcription Factors

Abstract

Glial cell line-derived neurotrophic factor (GDNF) transduces signal and promotes neurite outgrowths in diverse neurons through the interactions of GDNF family receptor alpha 1 (GFRalpha1) and other co-receptors including Ret receptor tyrosine kinase and NCAM. GFRalpha1 is alternatively spliced into two isoforms, GFRalpha1a and GFRalpha1b, with five amino acids difference. In this study, we found that both GFRalpha1a and GFRalpha1b were expressed in various human tissues. Interestingly, when stimulated with GDNF, GFRalpha1a but not GFRalpha1b promoted neurite outgrowth in neuroblastoma cells through the activations of ERK1/2, Rac1 and Cdc42. Remarkably, in cells co-expressing GFRalpha1a and GFRalpha1b, GDNF inhibited neurite outgrowths. The inhibitory activity of GFRalpha1b was dependent on RhoA and ROCK activation. Furthermore, GFRalpha1b but not GFRalpha1a activated Rho and various ROCK downstream effectors LIMK1/2, cofilin and MLC2. This study demonstrates the hitherto unrecognized roles of GFRalpha1 isoforms in the activation of distinct signaling pathways and in neurite outgrowths.

Published

2009

9. Carboxyl-Terminated Dendrimer-Coated Bioactive Interface for Protein Microarray: High-Sensitivity Detection of Antigen in Complex Biological Samples

Author

Gregory Stephanopoulos, Parayil Kumaran Ajikumar, Yew Chung Tang, Heng-Phon Too, Jin Kiat Ng, and Jim Yang Lee

Subjects

Proteomics, Dendrimers, Antibody microarray, Protein Array Analysis, Sensitivity and Specificity, Antibodies, Polyethylene Glycols, Propyleneimine, Mice, chemistry.chemical_compound, Adsorption, Cell Line, Tumor, Dendrimer, Polyamines, Electrochemistry, Animals, General Materials Science, Antigens, Spectroscopy, Cell-Free System, Chemistry, Drug discovery, Surfaces and Interfaces, Condensed Matter Physics, Biochemistry, Protein microarray, Biophysics

Abstract

Protein microarrays are promising tools that can potentially enable high throughput proteomic screening in areas such as disease diagnosis and drug discovery. A critical aspect in the development of protein microarrays is the optimization of the array's surface chemistry to achieve the high sensitivity required for detection of proteins in cell lysate and other complex biological mixtures. In the present study, a high-density antibody array with minimal nonspecific cellular protein adsorption was prepared using a glass surface coated with a poly(propyleneimine) dendrimer terminated with carboxyl group (PAMAM-COOH). The carboxyl-terminated dendrimer-modified surface has almost similar nonspecific cellular protein adsorption when compared to an inert PEG-modified surface. In addition, the multiple functional sites available for reaction on the dendrimer surface facilitated high-density immobilization of antibodies and efficient capture of bioanalytes. Various molecules were tested for their ability to block or deactivate the reactive carboxyl surface after antibody immobilization to further reduce the nonspecific binding. A short oligoethylene glycol (NH2-d4-PEG-COOH), was found to significantly improve the signal-to-noise ratio of the assay, resulting in higher sensitivity. The properties and functional qualities of the various surfaces were characterized by contact angle and AFM measurements. Nonspecific protein adsorption and protein immobilization as a function of dendrimer generations and sensitivity of antigen capturing from a buffer (1 pM) as well as from the complex cell lysate (10 pM) system were examined. Our detailed experimental studies demonstrated a facile method of preparing surfaces with high protein loading and low nonspecific protein binding for the development of high sensitivity protein microarrays.

Published

2007

10. A stem–loop-mediated reverse transcription real-time PCR for the selective detection and quantification of the replicative strand of an RNA virus

Author

Heng-Phon Too, Azlinda Anwar, and J. Thomas August

Subjects

Molecular Sequence Data, Biophysics, Genome, Viral, Viral Plaque Assay, Biology, Dengue virus, Virus Replication, medicine.disease_cause, Biochemistry, Virus, Mice, Cricetinae, Chlorocebus aethiops, Ribavirin, medicine, Animals, Humans, RNA Viruses, Vero Cells, Molecular Biology, Cells, Cultured, DNA Primers, Virus quantification, Mice, Inbred BALB C, Base Sequence, Reverse Transcriptase Polymerase Chain Reaction, RNA, RNA virus, Reverse Transcription, Cell Biology, Dengue Virus, Stem-loop, biology.organism_classification, Virology, Reverse transcriptase, Viral replication, Respiratory Syncytial Virus, Human, Nucleic Acid Conformation, RNA, Viral, West Nile virus

Abstract

A stem–loop-based method to quantify the replicative strand of a model system, dengue virus, with high specificity and sensitivity is described. The high specificity of this approach is achieved at two levels: the use of a reverse transcription primer folded into a stem–loop structure with optimal energetics and the use of specific PCR primers to the loop structure. This approach has exceptional specificity to the replicative RNA as compared with the genomic sequence (>10 5 -fold difference), with a detection sensitivity of 10 copies. The high correlation to the biological “gold standard” plaque assay, used to quantify infectious virus, renders this method a useful quantitative tool that can replace the time-consuming, labor-intensive, and low-throughput plaque-based assays. The method has been extended to the detection of replicative strands of other RNA viruses ( West Nile virus and human respiratory syncytial virus ) with similar results. This real-time PCR method is reliable, simple to perform, and easily adaptable to different targets. The ability to detect and rapidly quantify replicating viruses is an important step in the elucidation of pathogenesis and is also useful for the evaluation of drugs designed to inhibit viral replication.

Published

2006

11. The effects of particle size and surface coating on the cytotoxicity of nickel ferrite

Author

Gan Moog Chow, Heng-Phon Too, and Hong Yin

Subjects

Materials science, Cell Survival, Surface Properties, Biophysics, chemistry.chemical_element, Nanoparticle, Biocompatible Materials, Bioengineering, Nanotechnology, Ferric Compounds, Cell Line, Biomaterials, Mice, chemistry.chemical_compound, Coated Materials, Biocompatible, Microscopy, Electron, Transmission, X-Ray Diffraction, Pulmonary surfactant, Nickel, Cell Line, Tumor, Materials Testing, Animals, Particle Size, Micelles, Dose-Response Relationship, Drug, Microstructure, Surface coating, Oleic acid, chemistry, Chemical engineering, Mechanics of Materials, Ceramics and Composites, Magnetic nanoparticles, Particle size, Oleic Acid

Abstract

The safety and toxicity of nanoparticles are of growing concern despite their significant scientific interests and promising potentials in many applications. The properties of nanoparticles depend not only on the size but also the structure, microstructure and surface coating. These in turn are controlled by the synthesis and processing conditions. The dependence of cytotoxicity on particle size and on the presence of oleic acid as surfactant on nickel ferrite particles were investigated in vitro using the Neuro-2A cell line as a model. For nickel ferrite particles without oleic acid prepared by ball milling, cytotoxicity was independent of particle size within the given mass concentrations and surface areas accessible to the cells. For nickel ferrite particles coated with oleic acid prepared by the polyol method, the cytotoxicity significantly increased when one or two layers of oleic acid were deposited. Large particles (150+/-50 nm diameter) showed a higher cytotoxicity than smaller particles (10+/-3 nm diameter).

Published

2005

12. Polyethylene glycol modified polyethylenimine for improved CNS gene transfer: effects of PEGylation extent

Author

Ying Li, Jieming Zeng, Guping Tang, Shu Wang, Leilei Shi, Shujun Gao, Y.X. Ma, and Heng-Phon Too

Subjects

Male, Materials science, Cell Survival, Biophysics, Bioengineering, macromolecular substances, Polyethylene glycol, Gene delivery, Polyethylene Glycols, Biomaterials, chemistry.chemical_compound, Drug Delivery Systems, In vivo, PEG ratio, Animals, Polyethyleneimine, Tissue Distribution, Cells, Cultured, Injections, Spinal, Drug Implants, Neurons, Polyethylenimine, Gene Transfer Techniques, technology, industry, and agriculture, DNA, Transfection, Rats, Spinal Cord, chemistry, Biochemistry, Mechanics of Materials, Ceramics and Composites, PEGylation, Conjugate

Abstract

Poor solubility of polycation complexes with DNA is one drawback for their in vivo use as gene delivery systems. PEGylation often can improve the solubility of the complexes, minimize their aggregation and reduce their interaction with proteins in the physiological fluid. We investigated in vivo application of polyethylene glycol (PEG) modified polyethylenimine (PEI) for gene expression in the central nervous system. Varied numbers of linear PEG (2 kDa) were grafted to branched PEI (25 kDa) from the average number of PEG per one PEI macromolecule at 1-14.5. While higher degrees of PEG grafting did not improve gene expression, a PEI conjugate with one segment of PEG was able to mediate transgene expression in the spinal cord up to 11-fold higher than PEI homopolymer after intrathecal administration of its DNA complexes into the lumbar spinal cord subarachnoid space. Improved gene expression with this conjugate was observed as well in the brain after the lumbar injection. As assessed in in vitro studies, the PEI conjugate with a low degree of PEG grafting was able to reduce the size of polymer DNA complexes, prevent the aggregation of complexes, decrease the interactions of the complexes with serum proteins, counter the inhibition of serum to gene transfer, and enhance transfection efficiency, although not significant in affecting complex formation and reducing in vitro cell toxicity of PEI. The study provides the in vivo evidence that an appropriate degree of PEG modification is decisive in improving gene transfer mediated by PEGylated polymers.

Published

2003

13. Simultaneous extraction of total RNA and peptides from tissues: Application to tachykinins

Author

Heng-Phon Too and John E. Maggio

Subjects

Male, Preprotachykinin, Physiology, Substance P, Biology, Kidney, Polymerase Chain Reaction, Biochemistry, Rats, Sprague-Dawley, Cellular and Molecular Neuroscience, chemistry.chemical_compound, Endocrinology, Tachykinins, Gene expression, Methods, Animals, Northern blot, Chromatography, High Pressure Liquid, Brain Chemistry, Messenger RNA, Chromatography, Extraction (chemistry), RNA, Rats, Liver, Spinal Cord, chemistry, Female, RNA extraction, Peptides, DNA

Abstract

Methods for extraction and isolation of intact RNA are often laborious, time consuming, and preclude the direct analysis of peptides. Similarly, the conditions for extraction and isolation of peptides are unsuitable for the isolation of intact RNA. Thus, to study changes in the levels of neuropeptides and gene expression of the corresponding mRNAs, separate procedures are required. A simple and rapid method for the simultaneous extraction of RNA and peptides from tissues is described. RNA and peptides are extracted with guanidinium isothiocyanate, followed by delipidation, and peptides are isolated by a simple solid-phase extraction procedure. RNA is isolated by differentially partitioning DNA into an organic phase, followed by precipitation with ethanol. The RNA and peptides isolated by this method are of high yield and quality. Furthermore, this method for RNA isolation is successful and efficient, even with tissues that proved recalcitrant with other procedures, and allows the simultaneous processing of multiple samples. We describe the successful application of this procedure for measuring tachykinins and the corresponding preprotachykinin A mRNA from tissues. Extraction of neuropeptide K, a 36-mer tachykinin, was dramatically more efficient with the present method than other methods in common use.

Published

1995

14. PTEN/Akt signaling controls mitochondrial respiratory capacity through 4E-BP1

Author

Heng-Phon Too, Hwee Ying Lim, Kim Ping Wong, Chong Kiat Goo, Qin Shi Ho, and Marie-Veronique Clement

Subjects

Morpholines, lcsh:Medicine, Gene Expression, Cell Cycle Proteins, Mice, Transgenic, Mitochondrion, Bioenergetics, Biochemistry, Membrane Potentials, Electron Transport Complex IV, Mice, Adenosine Triphosphate, Molecular Cell Biology, Akt Signaling Cascade, PTEN, Animals, NRF1, Gene Silencing, Enzyme Inhibitors, lcsh:Science, Protein kinase B, Biology, PI3K/AKT/mTOR pathway, Cells, Cultured, Adaptor Proteins, Signal Transducing, Regulation of gene expression, Multidisciplinary, biology, lcsh:R, PTEN Phosphohydrolase, Tricarboxylic Acids, TFAM, Fibroblasts, Phosphoproteins, Molecular biology, Signaling Cascades, Mitochondria, Enzymes, Metabolism, Chromones, Protein Biosynthesis, biology.protein, Phosphorylation, lcsh:Q, Protein Translation, Proto-Oncogene Proteins c-akt, Research Article, Signal Transduction

Abstract

Akt, a serine/threonine kinase has been shown to stimulate glycolysis in cancer cells but its role in mitochondrial respiration is unknown. Using PTEN-knockout mouse embryonic fibroblasts (MEF(PTEN-/-)) with hyper-activated Akt as a cell model, we observed a higher respiratory capacity in MEF(PTEN-/-) compared to the wildtype (MEF(WT)). The respiratory phenotype observed in MEF(PTEN-/-) was reproduced in MEF(WT) by gene silencing of PTEN which substantiated its role in regulating mitochondrial function. The increased activities of the respiratory complexes (RCs) I, III and IV were retained in the same relative proportions as those present in MEF(WT), alluding to a possible co-ordinated regulation by PTEN/Akt. Using LY294002 (a PI3K inhibitor) and Akt inhibitor IV, we showed that the regulation of enzyme activities and protein expressions of the RCs was dependent on PI3K/Akt. There was insignificant difference in the protein expressions of mitochondrial transcription factor: peroxisome proliferator-activated receptor gamma coactivator 1-alpha (PGC-1α) and its downstream targets, the nuclear respiratory factor 1 (NRF-1) and mitochondrial transcription factor A (mtTFA) between MEF(PTEN-/-) and MEF(WT). Similarly, mRNA levels of the same subunits of the RCs detected in Western blots were not significantly different between MEF(PTEN-/-) and MEF(WT) suggesting that the regulation by Akt on mitochondrial function was probably not via gene transcription. On the other hand, a decrease of total 4E-BP1 with a higher expression of its phosphorylated form relative to total 4E-BP1 was found in MEF(PTEN-/-), which inferred that the regulation of mitochondrial respiratory activities by Akt was in part through this protein translation pathway. Notably, gene silencing of 4E-BP1 up-regulated the protein expressions of all RCs and the action of 4E-BP1 appeared to be specific to these mitochondrial proteins. In conclusion, PTEN inactivation bestowed a bioenergetic advantage to the cells by up-regulating mitochondrial respiratory capacity through the 4E-BP1-mediated protein translation pathway.

Published

2012

15. Cyclic AMP signalling through PKA but not Epac is essential for neurturin-induced biphasic ERK1/2 activation and neurite outgrowths through GFRα2 isoforms

Author

Qing 'En Lim, Yung Hou Wong, Heng-Phon Too, Guoqiang Wan, and Lihan Zhou

Subjects

Receptor complex, Glial Cell Line-Derived Neurotrophic Factor Receptors, Neurite, Cell Survival, MAP Kinase Signaling System, Neurturin, Blotting, Western, CREB, Real-Time Polymerase Chain Reaction, Transfection, Neurotrophic factors, Cell Line, Tumor, Glial cell line-derived neurotrophic factor, Cyclic AMP, Neurites, Animals, Humans, Protein Isoforms, Phosphorylation, Mitogen-Activated Protein Kinase 3, biology, Proto-Oncogene Proteins c-ret, Cell Biology, Cyclic AMP-Dependent Protein Kinases, Cell biology, Acetylcysteine, Erythromycin, Nerve Regeneration, Rats, Biochemistry, Gene Expression Regulation, biology.protein, GDNF Family Receptor Alpha-2, GDNF family of ligands, Signal Transduction

Abstract

Cyclic AMP (cAMP) and neurotrophic factors are known to interact closely to promote neurite outgrowth and neuronal regeneration. Glial cell line-derived neurotrophic factor (GDNF) and its family member neurturin (NTN) transduce signal through a multi-component receptor complex consisting of GDNF family receptor alpha 2 (GFRα2) and Ret receptor tyrosine kinase. Neurons from GFRα2-deficient mice do not promote axonal initiation when stimulated by NTN, consistent with the role of GFRα2 in neuronal outgrowth. Multiple alternatively spliced isoforms of GFRα2 are known to be expressed in the nervous system. GFRα2a and GFRα2c but not GFRα2b promoted neurite outgrowth. It is currently unknown if cAMP signalling is differentially regulated by these isoforms. In this study, NTN activation of GFRα2a and GFRα2c but not GFRα2b induced biphasic ERK1/2 activation and phosphorylation of the major cAMP target CREB. Interestingly, inhibition of cAMP signalling significantly impaired GFRα2a and GFRα2c-mediated neurite outgrowth while cAMP agonists cooperated with GFRα2b to induce neurite outgrowth. Importantly, the specific cAMP effector PKA but not Epac was essential for NTN-induced neurite outgrowth, through transcription and translation-dependent activation of late phase ERK1/2. Taken together, these results not only demonstrated the essential role of cAMP-PKA signalling in NTN-induced biphasic ERK1/2 activation and neurite outgrowth, but also suggested cAMP-PKA signalling as a hitherto unrecognized underlying mechanism contributing to the differential neuritogenic activities of GFRα2 isoforms.

Published

2011

16. Mitochondrial localized STAT3 is involved in NGF induced neurite outgrowth

Author

Heng-Phon Too and Lihan Zhou

Subjects

STAT3 Transcription Factor, Neurite, lcsh:Medicine, Biology, Mitochondrion, Bioinformatics, PC12 Cells, Signaling Pathways, Mediator, Nerve Growth Factor, Molecular Cell Biology, Neurites, Animals, STAT3, lcsh:Science, Multidisciplinary, Neuronal Morphology, lcsh:R, Mitochondria, Rats, Cell biology, Nerve growth factor, Cellular Neuroscience, biology.protein, STAT protein, Phosphorylation, lcsh:Q, Molecular Neuroscience, Neural development, Research Article, Signal Transduction, Neuroscience

Abstract

Background Signal transducer and activator of transcription 3 (STAT3) plays critical roles in neural development and is increasingly recognized as a major mediator of injury response in the nervous system. Cytokines and growth factors are known to phosphorylate STAT3 at tyrosine705 with or without the concomitant phosphorylation at serine727, resulting in the nuclear localization of STAT3 and subsequent transcriptional activation of genes. Recent evidence suggests that STAT3 may control cell function via alternative mechanisms independent of its transcriptional activity. Currently, the involvement of STAT3 mono-phosphorylated at residue serine727 (P-Ser-STAT3) in neurite outgrowth and the underlying mechanism is largely unknown. Principal Findings In this study, we investigated the role of nerve growth factor (NGF) induced P-Ser-STAT3 in mediating neurite outgrowth. NGF induced the phosphorylation of residue serine727 but not tyrosine705 of STAT3 in PC12 and primary cortical neuronal cells. In PC12 cells, serine but not tyrosine dominant negative mutant of STAT3 was found to impair NGF induced neurite outgrowth. Unexpectedly, NGF induced P-Ser-STAT3 was localized to the mitochondria but not in the nucleus. Mitochondrial STAT3 was further found to be intimately involved in NGF induced neurite outgrowth and the production of reactive oxygen species (ROS). Conclusion Taken together, the findings herein demonstrated a hitherto unrecognized novel transcription independent mechanism whereby the mitochondria localized P-Ser-STAT3 is involved in NGF induced neurite outgrowth.

Published

2011

17. A specific isoform of glial cell line-derived neurotrophic factor family receptor alpha 1 regulates RhoA expression and glioma cell migration

Author

Guoqiang, Wan and Heng-Phon, Too

Subjects

Glial Cell Line-Derived Neurotrophic Factor Receptors, Microscopy, Confocal, Reverse Transcriptase Polymerase Chain Reaction, Blotting, Western, Fluorescent Antibody Technique, Glioma, Transfection, Rats, Isomerism, Cell Movement, Animals, Neoplasm Invasiveness, Glial Cell Line-Derived Neurotrophic Factor, RNA, Small Interfering, rhoA GTP-Binding Protein, Neural Cell Adhesion Molecules, Cell Division

Abstract

Malignant gliomas are highly invasive neuroepithelial tumors where the tendency to invade and migrate away from the primary tumor mass is thought to be a leading cause of tumor recurrence and treatment failures. Autocrine signals produced by secreted factors that signal through receptors on the tumor are known to contribute to the invasiveness. Glial cell line-derived neurotrophic factor and GDNF family receptor alpha 1 (GFRα1) are over-expressed in human gliomas. We have previously reported that human gliomas express high levels of GFRα1b, an alternatively spliced isoform of GFRα1. However, the functional significance of GFRα1b in glioma behaviors is currently unknown. In this study, we have designed isoform-specific small-interfering RNA to knockdown the highly homologous GFRα1a or GFRα1b isoform efficiently in malignant C6 glioma cells. Unexpectedly, the knockdown of GFRα1b but not GFRα1a induced cell elongation and inhibited C6 cell migration and invasion in vitro. In addition, GFRα1b was found to regulate the expression of RhoA small GTPase, which was required for migration of C6 cells. The decreases in RhoA expression and cell migration after GFRα1b knockdown were attenuated by small-interfering RNA -resistant GFRα1b but not GFRα1a, further demonstrating the specific role of GFRα1b in glioma migration. Interestingly, the knockdown of NCAM but not receptor tyrosine kinase Ret resulted in the reduction of RhoA expression and C6 cell migration. Taken together, these unanticipated results indicate that GFRα1b is involved in glioma migration through glial cell line-derived neurotrophic factor -GFRα1b-NCAM signaling complex and modulation of RhoA expression.

Published

2010

18. Identification and validation of reference genes for expression studies in a rat model of neuropathic pain

Author

Heng-Phon Too, Hee Kit Wong, Kai Yang, Guoqiang Wan, Lihan Zhou, Qing 'En Lim, and Bei Ping He

Subjects

Male, Ribosomal Protein L3, Biophysics, Pain, Biology, Bioinformatics, Biochemistry, Rats, Sprague-Dawley, Reference Values, Reference genes, Gene expression, Animals, Trauma, Nervous System, Molecular Biology, Gene, Glyceraldehyde 3-phosphate dehydrogenase, Oligonucleotide Array Sequence Analysis, Gene Expression Profiling, Cell Biology, Housekeeping gene, Rats, Gene expression profiling, Disease Models, Animal, Neuropathic pain, biology.protein, DNA microarray

Abstract

Neuropathic pain is triggered by damage to or as a result of the dysfunction of the somatosensory nervous system. Gene expression profiling using DNA microarray and real-time PCR have emerged as powerful tools for the elucidation of pain-specific pathways and identification of candidate biomarkers and therapeutic targets. Proper normalization of the gene expression data with stable reference genes is a prerequisite to obtaining accurate gene expression changes. We have evaluated the stability of six candidate reference genes which include three commonly used housekeeping genes (ACTB, GAPDH and HMBS) and three ribosomal protein genes (RPL3, RPL19 and RPL29) using real-time PCR in a rat model of neuropathic pain. Unexpectedly, ACTB but not GAPDH was stably expressed. In addition, we have identified RPL29 and RPL3 as novel reference genes. Normalization of expression data using GAPDH or HMBS led to overestimation of transcriptional changes. Using RPL29/RPL3/ACTB as reference genes, a number of transcripts were found to be specifically and significantly regulated in injured dorsal root ganglia. These genes may contribute to the development of neuropathic pain pathology and may serve as candidate biomarkers for potential diagnosis.

Published

2010

19. Normalization with genes encoding ribosomal proteins but not GAPDH provides an accurate quantification of gene expressions in neuronal differentiation of PC12 cells

Author

Lihan Zhou, Guoqiang Wan, Heng-Phon Too, and Qing-En Lim

Subjects

Ribosomal Proteins, Candidate gene, lcsh:QH426-470, lcsh:Biotechnology, Biology, PC12 Cells, Reference genes, lcsh:TP248.13-248.65, Gene expression, Genetics, Animals, Gene, Oligonucleotide Array Sequence Analysis, Regulation of gene expression, Reverse Transcriptase Polymerase Chain Reaction, Microarray analysis techniques, Gene Expression Profiling, Glyceraldehyde-3-Phosphate Dehydrogenases, Reference Standards, Rats, Housekeeping gene, Cell biology, lcsh:Genetics, DNA microarray, Research Article, Biotechnology

Abstract

Background Gene regulation at transcript level can provide a good indication of the complex signaling mechanisms underlying physiological and pathological processes. Transcriptomic methods such as microarray and quantitative real-time PCR require stable reference genes for accurate normalization of gene expression. Some but not all studies have shown that housekeeping genes (HGKs), β-actin (ACTB) and glyceraldehyde-3-phosphate dehydrogenase (GAPDH), which are routinely used for normalization, may vary significantly depending on the cell/tissue type and experimental conditions. It is currently unclear if these genes are stably expressed in cells undergoing drastic morphological changes during neuronal differentiation. Recent meta-analysis of microarray datasets showed that some but not all of the ribosomal protein genes are stably expressed. To test the hypothesis that some ribosomal protein genes can serve as reference genes for neuronal differentiation, a genome-wide analysis was performed and putative reference genes were identified based on stability of expressions. The stabilities of these potential reference genes were then analyzed by reverse transcription quantitative real-time PCR in six differentiation conditions. Results Twenty stably expressed genes, including thirteen ribosomal protein genes, were selected from microarray analysis of the gene expression profiles of GDNF and NGF induced differentiation of PC12 cells. The expression levels of these candidate genes as well as ACTB and GAPDH were further analyzed by reverse transcription quantitative real-time PCR in PC12 cells differentiated with a variety of stimuli including NGF, GDNF, Forskolin, KCl and ROCK inhibitor, Y27632. The performances of these candidate genes as stable reference genes were evaluated with two independent statistical approaches, geNorm and NormFinder. Conclusions The ribosomal protein genes, RPL19 and RPL29, were identified as suitable reference genes during neuronal differentiation of PC12 cells, regardless of the type of differentiation conditions. The combination of these two novel reference genes, but not the commonly used HKG, GAPDH, allows robust and accurate normalization of differentially expressed genes during PC12 differentiation.

Published

2010

20. Glial cell line-derived neurotrophic factor and neurturin inhibit neurite outgrowth and activate RhoA through GFR alpha 2b, an alternatively spliced isoform of GFR alpha 2

Author

Heng-Phon Too and Li Foong Yoong

Subjects

Receptor complex, RHOA, Glial Cell Line-Derived Neurotrophic Factor Receptors, Neurite, Neurturin, Cell Line, Mice, Neurotrophic factors, Glial cell line-derived neurotrophic factor, Neurites, Animals, Humans, Protein Isoforms, Glial Cell Line-Derived Neurotrophic Factor, Cell Proliferation, biology, General Neuroscience, Articles, Molecular biology, Growth Inhibitors, Alternative Splicing, biology.protein, Neural cell adhesion molecule, rhoA GTP-Binding Protein, GDNF family of ligands

Abstract

The glial cell line-derived neurotrophic factor (GDNF) and neurturin (NTN) belong to a structurally related family of neurotrophic factors. NTN exerts its effect through a multicomponent receptor system consisting of the GDNF family receptor alpha2 (GFR alpha2), RET, and/or NCAM (neural cell adhesion molecule). GFR alpha2 is alternatively spliced into at least three isoforms (GFR alpha2a, GFR alpha2b, and GFR alpha2c). It is currently unknown whether these isoforms share similar functional and biochemical properties. Using highly specific and sensitive quantitative real-time PCR, these isoforms were found to be expressed at comparable levels in various regions of the human brain. When stimulated with GDNF and NTN, both GFR alpha2a and GFR alpha2c, but not GFR alpha2b, promoted neurite outgrowth in transfected Neuro2A cells. These isoforms showed ligand selectivity in MAPK (mitogen-activated protein kinase) [ERK1/2 (extracellular signal-regulated kinase 1/2)] and Akt signaling. In addition, the GFR alpha2 isoforms regulated different early-response genes when stimulated with GDNF or NTN. In coexpression studies, GFR alpha2b was found to inhibit ligand-induced neurite outgrowth by GFR alpha2a and GFR alpha2c. Stimulation of GFR alpha2b also inhibited the neurite outgrowth induced by GFR alpha1a, another member of the GFR alpha. Furthermore, activation of GFR alpha2b inhibited neurite outgrowth induced by retinoic acid and activated RhoA. Together, these data suggest a novel paradigm for the regulation of growth factor signaling and neurite outgrowth via an inhibitory splice variant of the receptor. Thus, depending on the expressions of specific GFR alpha2 receptor spliced isoforms, GDNF and NTN may promote or inhibit neurite outgrowth through the multicomponent receptor complex.

Published

2007

21. Establishing efficient siRNA knockdown in mouse embryonic stem cells

Author

Heng-Phon Too, Andre Choo, Steve Oh, Nai-dy Wang, and Stephen Chen

Subjects

Small interfering RNA, animal structures, Transcription, Genetic, viruses, Blotting, Western, Bioengineering, Biology, Transfection, Applied Microbiology and Biotechnology, Cell Line, Mice, RNA interference, Animals, RNA, Small Interfering, Embryonic Stem Cells, Gene knockdown, Reverse Transcriptase Polymerase Chain Reaction, fungi, RNA, General Medicine, Embryonic stem cell, Molecular biology, Cell culture, embryonic structures, Stem cell, Octamer Transcription Factor-3, Biotechnology

Abstract

FAM-labeled oligo dT (FAMdT) was utilized as a means to gauge efficient transfection of small nucleic acids into mouse embryonic stem cell (mESC) colonies. Using colonies grown overnight, transfection was restricted largely to the periphery of the colonies with only a 40% decrease in Oct-3/4 RNA transcript levels following cognate Oct-3/4, small interfering RNA (siRNA) delivery. However, transfection of mESC 4 h after seeding gave greater than 90% cells being successfully transfected based on quantitative real-time PCR detection of approximately 90% Oct-3/4 RNA transcript knockdown. This method provides an economical and efficient means by which to determine effective transfection conditions, and establish efficient siRNA knockdown of reportedly difficult to transfect cell lines such as mESC.

Published

2006

22. Tissue expression of alternatively spliced GFRalpha1, NCAM and RET isoforms and the distinct functional consequence of ligand-induced activation of GFRalpha1 isoforms

Author

Guoqiang Wan, Zhong Ni Peng, Li Foong Yoong, and Heng-Phon Too

Subjects

Gene isoform, Glial Cell Line-Derived Neurotrophic Factor Receptors, Microarray, Gene Expression, Ligands, Cell Line, Cellular and Molecular Neuroscience, Mice, Neurotrophic factors, Glial cell line-derived neurotrophic factor, Animals, Humans, Protein Isoforms, Tissue Distribution, Receptor, Extracellular Signal-Regulated MAP Kinases, Molecular Biology, Gene, Neural Cell Adhesion Molecules, Oligonucleotide Array Sequence Analysis, biology, Gene Expression Profiling, Proto-Oncogene Proteins c-ret, Transfection, Molecular biology, Alternative Splicing, nervous system, biology.protein, Neural cell adhesion molecule

Abstract

Glial-cell-line-derived neurotrophic factor (GDNF) exerts its effect through a multi-component receptor system consisting of GFRalpha1, RET and NCAM. Two highly homologous alternatively spliced GFRalpha1 isoforms (GFRalpha1a and GFRalpha1b) have previously been identified. In this study, isoform specific real-time PCR assays were used to quantify the expression levels of GFRalpha1, RET and NCAM isoforms in murine embryonic and adult tissues. The expression levels of GFRalpha1b were found to be comparable to that of GFRalpha1a in peripheral tissues. However, GFRalpha1a was the predominant isoform expressed in the whole brain. The co-expressions of GFRalpha1 and the co-receptors were developmentally regulated and differentially expressed in some tissues. Microarray analyses of GFRalpha1 isoforms transfected cells stimulated with NTN showed distinct and non-overlapping gene profiles. These observations are consistent with the emerging view that the combinatorial interactions of the spliced isoforms of GFRalpha, RET and NCAM may contribute to the pleiotropic biological responses.

Published

2005

23. Association behavior of biotinylated and non-biotinylated poly(ethylene oxide)-b-poly(2-(diethylamino)ethyl methacrylate)

Author

Heng-Phon Too, P. Ravi, Tan Jf, Hatton Ta, and Kam Chiu Tam

Subjects

Time Factors, Polymers and Plastics, Light, Cell Survival, Polymers, Radical polymerization, Bioengineering, Methacrylate, Micelle, Polyethylene Glycols, Biomaterials, chemistry.chemical_compound, Dynamic light scattering, Polymer chemistry, Materials Chemistry, Copolymer, Animals, Humans, Scattering, Radiation, Static light scattering, Biotinylation, Micelles, chemistry.chemical_classification, Ethylene oxide, Molecular Structure, Lasers, Polymer, Hydrogen-Ion Concentration, Nylons, chemistry, Potentiometry, Methacrylates

Abstract

Biotinylated and non-biotinylated copolymers of poly(ethylene oxide) (PEO) and poly(2-(diethylamino)ethyl methacrylate) (PDEAEMA) were synthesized by the atom transfer radical polymerization technique. The chemical compositions of the copolymers as determined by NMR are represented by PEO(113)PDEAEMA(70) and biotin-PEO(104)PDEAEMA(93), respectively. The aggregation behavior of these polymers in aqueous solutions at different pHs and ionic strengths was studied using a combination of potentiometric titration, dynamic light scattering, static light scattering, and transmission electron microscopy. Both PEO-b-PDEAEMA and biotin-PEO-b-PDEAEMA diblock copolymers form micelles at high pH with hydrodynamic radii (R(h)) of about 19 and 23 nm, respectively. At low pH, the copolymers are dispersed as unimers in solution with R(h) values of about 6-7 nm. However, at a physiological salt concentration (c(s)) of about 0.16 M NaCl and a pH of 7-8, the copolymers form large loosely packed Gaussian chains, which were not present at the low c(s) of 0.001 M NaCl. The critical micelle concentrations (cmc's) and the cytotoxicities of the copolymers were investigated to determine a suitable polymer concentration range for future biological applications. Both PEO-b-PDEAEMA and biotin-PEO-b-PDEAEMA diblock copolymers possess identical cmc values of about 0.0023 mg/g, while the cytotoxicity test indicated that the copolymers are not toxic up to 0.05 mg/g (83% cell survival at this concentration).

Published

2005

24. A synthetic peptide containing loop 4 of nerve growth factor for targeted gene delivery

Author

Shu Wang, Heng-Phon Too, Elizabeth S. E. Luo, Yuexia Ma, and Jieming Zeng

Subjects

animal structures, Cell Survival, Genetic Vectors, Tropomyosin receptor kinase B, Biology, Tropomyosin receptor kinase A, Gene delivery, PC12 Cells, Culture Media, Serum-Free, Mice, Cerebellum, Drug Discovery, Gene expression, Nerve Growth Factor, Genetics, Low-affinity nerve growth factor receptor, Animals, Receptor, trkA, Molecular Biology, Genetics (clinical), Cerebral Cortex, Neurons, Reporter gene, Gene Transfer Techniques, Transfection, Molecular biology, Rats, Nerve growth factor, nervous system, NIH 3T3 Cells, Molecular Medicine, Peptides, Neuroglia, Signal Transduction

Abstract

Background Gene delivery vectors that restrict the expression of a therapeutic gene to a particular type of cells are critical to gene therapy in a complex structure, such as the central nervous system. We constructed a nonviral vector for targeted gene transfer to cells expressing nerve growth factor (NGF) receptor TrkA. Methods and results The vector was a synthetic chimeric peptide composed of a targeting moiety derived from NGF loop 4 and a DNA-binding moiety of 10 lysine residues. The peptide activated signal transduction pathways of the NGF receptor TrkA in PC12 cells and supported the survival of the cells after serum deprivation. After forming complexes with plasmid DNA, the peptide dose-dependently increased reporter gene expression in PC12 cells, which could be inhibited by excess NGF. The peptide-mediated gene expression was not affected in PC12 cells by co-incubation with a blocking antibody against the low-affinity NGF receptor p75 and was significantly enhanced in NIH3T3 cells stably transfected with TrkA cDNA, suggesting the involvement of the high-affinity NGF receptor TrkA without the participation of p75. Moreover, the peptide did not assist gene transfer in TrkA-poor, but TrkB- and/or TrkC-positive primary cerebellar granule neurons and primary cortical glial cells. Conclusions The chimeric peptide reported will be useful in gene delivery to and gene therapy of the nervous system and other tissues/organs with cells expressing TrkA. Copyright © 2004 John Wiley & Sons, Ltd.

Published

2004

25. Preprotachykinin-A and substance P receptor (NK1) gene expression in rat astrocytes in vitro

Author

Derek R. Marriott, Graham P. Wilkin, and Heng-Phon Too

Subjects

Male, medicine.medical_specialty, Gene Expression, Substance P, Biology, Polymerase Chain Reaction, Substance-P Receptor, chemistry.chemical_compound, Tachykinins, Internal medicine, Gene expression, medicine, Animals, RNA, Messenger, Protein Precursors, Receptor, Autocrine signalling, General Neuroscience, Brain, Receptors, Neurokinin-1, Molecular biology, Rats, medicine.anatomical_structure, Endocrinology, chemistry, Astrocytes, Interleukin-21 receptor, Neuroglia, Female, Astrocyte

Abstract

The presence of mRNA transcripts coding for preprotachykinin-A and the substance P receptor in cultured astrocytes is demonstrated by a combination of reverse transcription/polymerase chain reaction (PCR) and Southern blotting. These findings showed that astrocytes in culture are capable of synthesing both the precursor of substance P (preprotachykinin-A) and the cognate receptor, substance P receptor (NK1). The simultaneous presence of both the ligand (substance P) and the receptor (NK1) may indicate an autocrine nature of astrocyte communication.

Published

1994

26. Crystallization and preliminary X-ray study of recombinant betaine-homocysteine S-methyltransferase from rat liver

Author

Francisco Garrido, Beatriz González, Julia Sanz-Aparicio, Tom L. Blundell, Heng Phon Too, and María A. Pajares

Subjects

Homocysteine, Stereochemistry, Protein Conformation, Betaine—homocysteine S-methyltransferase, Crystallography, X-Ray, law.invention, Dimethylglycine, chemistry.chemical_compound, Betaine, Structural Biology, law, Animals, DNA Primers, chemistry.chemical_classification, Methionine, Base Sequence, General Medicine, Methyltransferases, Recombinant Proteins, Rats, Enzyme, chemistry, Biochemistry, Betaine-Homocysteine S-Methyltransferase, Liver, Recombinant DNA, Crystallization, Function (biology)

Abstract

4 páginas, 4 figuras, 1 tabla.-- et al., Betaine-homocysteine S-methyltransferase is one of the three enzymes involved in homocysteine catabolism. It uses betaine as the methyl donor to convert homocysteine into methionine, also producing dimethylglycine. Recombinant BHMT from rat liver was crystallized by the vapour-diffusion method in both native and seleniomethionyl-labelled forms. Crystals belong to space group P21, with unit-cell parameters a = 57.8, b = 149.3, c = 96.2 Å, β= 92.9°. Data from native, seleniomethionine-labelled and two heavy-atom derivatives were collected using synchrotron sources. Self-rotation function and sedimentation-velocity experiments suggest that the enzyme is tetrameric with 222 symmetry.

Published

2002

27. Quantification of mouse glial cell-line derived neurotrophic factor family receptor alpha 2 alternatively spliced isoforms by real time detection PCR using SYBR Green I

Author

Heng-Phon Too, G.M. Sia, and Y.W. Wong

Subjects

Gene isoform, Glial Cell Line-Derived Neurotrophic Factor Receptors, Neurturin, Diamines, Polymerase Chain Reaction, chemistry.chemical_compound, Mice, Neurotrophic factors, Proto-Oncogene Proteins, Glial cell line-derived neurotrophic factor, Animals, Drosophila Proteins, Protein Isoforms, Benzothiazoles, Nerve Growth Factors, RNA, Messenger, Organic Chemicals, DNA Primers, Fluorescent Dyes, Brain Chemistry, Neurons, biology, urogenital system, General Neuroscience, Proto-Oncogene Proteins c-ret, Brain, Receptor Protein-Tyrosine Kinases, Reproducibility of Results, Molecular biology, Alternative Splicing, Real-time polymerase chain reaction, chemistry, Mutation, biology.protein, SYBR Green I, Quinolines, Oligonucleotide Probes, GDNF Family Receptor Alpha-2

Abstract

Neurturin (NTN) belongs to the glial cell-line derived neurotrophic factor (GDNF) family of growth factors. Both NTN and GDNF have been shown to potently prevent the degeneration of dopaminergic neuron in vitro and in vivo. The GDNF family receptor alpha 2 (GFR alpha-2) is the preferred receptor for NTN. In addition to the known full-length isoform (GFR alpha-2a), we have previously reported the isolation of two novel alternatively spliced isoforms (GFR alpha-2b and GFR alpha-2c). All three isoforms are expressed in all mammalian tissues examined, including human fetal brain. However, the expression levels of these isoforms have yet to be quantified. In this report, we have developed a real time polymerase chain reaction (PCR) detection method using SYBR Green I to detect the expression levels of the three splice variants (GFR alpha-2a, GFR alpha-2b and GFR alpha-2c). Of the three isoforms, GFR alpha-2a was found to be the most abundant receptor expressed in the whole murine brain. The real time PCR detection method using SYBR Green I developed in this report can be used to unambiguously quantitate expression levels of the GFR alpha-2 isoforms and can be extended to the quantitation of other alternatively spliced isoforms.

Published

2002

28. Creation of nanostructures by interference lithography for modulation of cell behavior

Author

Raj Rajagopalan, Wee Kiong Choi, Chang Quan Lai, M. K. Dawood, Minmin Zhu, Baojun Li, Lihan Zhou, Heng-Phon Too, K. C. Leong, H. Cheng, and Guoqiang Wan

Subjects

Silicon, Materials science, Nanostructure, Surface Properties, Green Fluorescent Proteins, chemistry.chemical_element, Nanotechnology, Nanostructures, Interference lithography, Mice, Resins, Synthetic, chemistry, Modulation, Cell Line, Tumor, Animals, General Materials Science, Nanoscopic scale

Abstract

Emerging evidence of the striking differences that can be induced in the behavior of biological cells through topographical modulation of physically and chemically patterned nanostructured surfaces provides a great impetus for developing novel cellular-scale and sub-cellular-scale nanopatterned substrates and for employing them for exciting new applications in life and medical sciences and biotechnology. However, the lack of availability of cost-effective, large-surface-area nanofabricated substrates of appropriate dimensions and features has proved to be a major impediment for research in this area. Here, we demonstrate a simple and cost-effective method based on interference lithography to produce spatially precise and wide-surface-coverage silicon- and polymer-based nanostructures to study how cells react to nanoscale structures or surfaces.

Published

2011

29. Immunocytochemical localization of neuromedin K (neurokinin B) in rat spinal ganglia and cord

Author

Heng-Phon Too and John E. Maggio

Subjects

Male, Pathology, medicine.medical_specialty, Cord, Physiology, Neurokinin B, Neurokinin A, Central nervous system, Immunocytochemistry, Neuropeptide, Substance P, Biology, Biochemistry, Cellular and Molecular Neuroscience, chemistry.chemical_compound, Endocrinology, Ganglia, Spinal, medicine, Animals, Tissue Distribution, Rats, Inbred Strains, Anatomy, Spinal cord, Immunohistochemistry, Rats, medicine.anatomical_structure, chemistry, Spinal Cord, Female

Abstract

Specific antisera directed against substance P and neuromedin K (neurokinin B) have been used in double-label immunofluorescence studies to unambiguously localize these two neuropeptides of the tachykinin family in single tissue sections of rat spinal cord and dorsal root ganglia. Substance P-like immunoreactivity (SPLI) is present but neuromedin K-like immunoreactivity (NMKLI) is undetectable in dorsal root ganglia. Both peptides are present in the spinal cord, but NMKLI is largely restricted to the dorsal gray while SPLI shows a broader distribution. In the spinal gray, NMKLI coexists with SPLI in some, but not all, fibers. While substance P in the dorsal spinal cord is largely of primary afferent origin, neuromedin K appears to originate largely from intrinsic spinal neurons.

Published

1991

30. Calcitonin Gene-related Polypeptide as a Mediator of the Neurogenic Ocular Injury Response

Author

Heng-Phon Too, John M Butler, William G. Unger, Julia M. Polak, M. A. Ghatei, Keith W. Ennis, Giorgio Terenghi, Steven R. Bloom, and Shu Qi Zhang

Subjects

Male, medicine.medical_specialty, genetic structures, Calcitonin Gene-Related Peptide, Guinea Pigs, Neuropeptide, Substance P, Calcitonin gene-related peptide, Eye, Guinea pig, chemistry.chemical_compound, Internal medicine, medicine, Animals, Pharmacology (medical), Trigeminal Nerve, Pharmacology, Afferent Pathways, Chemistry, Neuropeptides, Nociceptors, Rats, Inbred Strains, Uvea, eye diseases, Rats, Antidromic, Ganglion, Ophthalmology, Endocrinology, medicine.anatomical_structure, Calcitonin, Female, Rabbits, sense organs

Abstract

Calcitonin gene-related polypeptide (CGRP) has been localised immunochemically within the rat and guinea pig anterior uvea to nerve fibres of trigeminal origin. As with substance P (1-3) the level of CGRP in the iris-ciliary body is depleted after thermal damage to the Gasserian ganglion and elevated in chronically sympathectically denervated eyes. Unlike substance P, a potent pupillary constrictor (4,5), CGRP has no notable miotic action, but does, however, cause an elevation of the intraocular pressure (IOP) accompanied by disruption of the blood-aqueous barrier. It is proposed that the diverse actions of these two sensory neuropeptides conjointly mediate the antidromic ocular injury response.

Published

1985

31. Presence and actions of vasopressin-like peptides in the rabbit anterior uvea

Author

W.G. Unger, K. Todd, A. Horn, M.R. Hanley, Heng-Phon Too, and Stafford L. Lightman

Subjects

Receptors, Vasopressin, Vasopressin, medicine.medical_specialty, Vasopressins, Physiology, Inositol Phosphates, Clinical Biochemistry, Iris sphincter muscle, Iris, Neuropeptide, Biology, Eye, Biochemistry, Cornea, Angiotensin Receptor Antagonists, Cellular and Molecular Neuroscience, Endocrinology, Ciliary body, Internal medicine, medicine, Animals, Trigeminal Nerve, Iris (anatomy), Vasopressin receptor, Denervation, urogenital system, Ciliary Body, Arginine Vasopressin, medicine.anatomical_structure, Rabbits, hormones, hormone substitutes, and hormone antagonists

Abstract

The presence of vasopressin-like immunoreactivity (VP-IR) in the rabbit eye was demonstrated by radioimmunoassay. Trigeminal nerve denervation resulted in a significant and selective decrease in the levels of VP-IR in the iris sphincter muscle and the cornea. The isolated iris sphincter muscle contracted in response to low concentrations of [Arg8]vasopressin (AVP) and related peptides. The V1 vasopressin receptor antagonist, d(CH2)5Tyr(Me)AVP, potently inhibited the contractile responses to AVP. AVP was found to induce an increase in the accumulation of inositol phosphates in the iris sphincter muscle but not in the dilator/ciliary body preparation in vitro. The present investigation demonstrates the presence of VP-IR in the rabbit eye and that this substance may be another sensory nerve-derived mediator acting on specific target sites in the anterior uvea.

Published

1989

32. Heterogeneity of tachykinin-like immunoreactive peptides in rat spinal cord and dorsal root ganglia

Author

Heng-Phon Too, Jose L. Cordova, and John E. Maggio

Subjects

Male, medicine.medical_specialty, Physiology, Central nervous system, Radioimmunoassay, Neuropeptide, Substance P, Cross Reactions, Biology, Substance K, Biochemistry, High-performance liquid chromatography, Cellular and Molecular Neuroscience, chemistry.chemical_compound, Endocrinology, Ganglia, Spinal, Tachykinins, Internal medicine, medicine, Animals, Chromatography, High Pressure Liquid, Rats, Inbred Strains, Spinal cord, Rats, medicine.anatomical_structure, Spinal Cord, chemistry, Female, Neurokinin B

Abstract

The concentrations of tachykinins in rat spinal cord and dorsal root ganglia (DRGs) were measured using a combination of high performance liquid chromatography (HPLC) and radioimmunoassays (RIAs). Substance P-like immunoreactivity (SPLI) was found to be significantly higher than either substance K-like immunoreactivity (SKLI) or neuromedin K-like immunoreactivity (NMKLI) in both tissues. In the spinal cord, the concentration of SKLI was comparable to that of NMKLI. In DRGs, NMKLI is present at concentrations much lower than those of SKLI or SPLI. In addition to immunoreactive components co-eluting with the three mammalian tachykinins SP, SK and NMK, analyses using reverse-phase HPLC revealed an immunoreactive peak co-eluting with the C-terminal octapeptide of SK (SK3-10), and a yet to be identified peak eluting before SK. This study also demonstrates the use of a novel and highly specific RIA for NMK to measure NMKLI without the need of reverse-phase HPLC.

Published

1989

33. Substance P receptor binding sites are expressed by glia in vivo after neuronal injury

Author

Mark Catton, Steven R. Vigna, Patrick W. Mantyh, Christian G. Boehmer, Harry V. Vinters, John E. Maggio, Donald J. Johnson, and Heng-Phon Too

Subjects

Male, medicine.medical_specialty, Substance P, Receptors, Cell Surface, Biology, Neurotransmission, Glial scar, chemistry.chemical_compound, Neurotransmitter receptor, Internal medicine, medicine, Animals, Neurotransmitter metabolism, Galanin, Receptor, Substance P receptor binding, Neurons, Multidisciplinary, Brain, Optic Nerve, Receptors, Neurokinin-1, Receptors, Neurotransmitter, Kinetics, Endocrinology, chemistry, nervous system, Rabbits, Neuroglia, Research Article

Abstract

In vitro studies have demonstrated that glia can express functional receptors for a variety of neurotransmitters. To determine whether similar neurotransmitter receptors are also expressed by glia in vivo, we examined the glial scar in the transected optic nerve of the albino rabbit by quantitative receptor autoradiography. Receptor binding sites for radiolabeled calcitonin gene-related peptide, cholecystokinin, galanin, glutamate, somatostatin, substance P, and vasoactive intestinal peptide were examined. Specific receptor binding sites for each of these neurotransmitters were identified in the rabbit forebrain but were not detected in the normal optic nerve or tract. In the transected optic nerve and tract, only receptor binding sites for substance P were expressed at detectable levels. The density of substance P receptor binding sites observed in this glial scar is among the highest observed in the rabbit forebrain. Ligand displacement and saturation experiments indicate that the substance P receptor binding site expressed by the glial scar has pharmacological characteristics similar to those of substance P receptors in the rabbit striatum, rat brain, and rat and canine gut. The present study demonstrates that glial cells in vivo express high concentrations of substance P receptor binding sites after transection of retinal ganglion cell axons. Because substance P has been shown to regulate inflammatory and immune responses in peripheral tissues, substance P may also, by analogy, be involved in regulating the glial response to injury in the central nervous system.

Published

1989

34. A novel radioimmunoassay for neuromedin K. I. Absence of neuromedin K-like immunoreactivity in guinea pig ileum and urinary bladder. II. Heterogeneity of tachykinins in guinea pig tissues

Author

Heng-Phon Too, John E. Maggio, and Jose L. Cordova

Subjects

Male, medicine.medical_specialty, Physiology, Neurokinin B, Clinical Biochemistry, Guinea Pigs, Urinary Bladder, Radioimmunoassay, Neuropeptide, Ileum, Substance P, Peptide hormone, Substance K, Biochemistry, Binding, Competitive, Guinea pig, Cellular and Molecular Neuroscience, chemistry.chemical_compound, Endocrinology, Internal medicine, Tachykinins, medicine, Animals, Tissue Distribution, medicine.anatomical_structure, chemistry

Abstract

A novel and highly specific radioimmunoassay for the tachykinin peptide neuromedin K (NMK, also known as neurokinin beta, neurokinin B) has been developed and used to determine the distribution of this peptide in extracts of guinea pig tissues. In addition to immunoreactive components coeluting with the 3 mammalian tachykinins, substance P (SP), substance K (SK) and NMK, analyses using reverse-phase HPLC revealed immunoreactive peaks coeluting with the C-terminal octapeptide of SK (SK-(3-10], an N-terminally extended form of SK (gamma-preprotachykinin-(72-92)amide), and a yet unidentified peak eluting before NMK in the extracts of guinea pig brain and spinal cord. In contrast to the other tachykinins, SP and SK, which were present in high concentrations in extracts of all peripheral and central tissues examined, NMK-like immunoreactivity was detected only in extracts of central tissues. NMK-like immunoreactivity was not detected in extracts of terminal ileum and urinary bladder.

Published

1989