Your search keyword '"Masaaki Kitada"' showing total 110 results

51. The expression of PLP/DM-20 mRNA is restricted to the oligodendrocyte-lineage cells in the adult rat spinal cord

Author

Mari Dezawa, Kazuya Takeda, and Masaaki Kitada

Subjects

0301 basic medicine, Male, Histology, Proteolipid protein 1, Population, chemical and pharmacologic phenomena, In situ hybridization, Biology, OLIG2, 03 medical and health sciences, 0302 clinical medicine, immune system diseases, medicine, Animals, Cell Lineage, RNA, Messenger, Rats, Wistar, education, Myelin Proteolipid Protein, Molecular Biology, In Situ Hybridization, Messenger RNA, education.field_of_study, Oligodendrocyte differentiation, Cell Biology, Molecular biology, Oligodendrocyte, nervous system diseases, Myelin proteolipid protein, Rats, Medical Laboratory Technology, Oligodendroglia, 030104 developmental biology, medicine.anatomical_structure, nervous system, Spinal Cord, lipids (amino acids, peptides, and proteins), 030217 neurology & neurosurgery

Abstract

Proteolipid protein (PLP) is the major component of myelin; its gene encodes two major splicing variants: PLP and DM-20. Compared with PLP, DM-20 lacks the amino acids encoded by exon IIIb. The expression of PLP/DM-20 in cells outside the oligodendrocyte-lineage is unclear. To address this issue, we analyzed the detailed expression pattern of PLP/DM-20 mRNA in the adult rat spinal cord by in situ hybridization (ISH) with a cRNA probe complementary to DM-20 mRNA, which has been used to detect both PLP and DM-20 both mRNA. ISH did not label the cells expressing NeuN nor glial fibrillary acidic protein but detected those expressing Olig2, indicating that PLP/DM-20 mRNA are expressed only in oligodendrocyte-lineage cells. This cell population was expected to contain NG2-expressing oligodendrocyte precursor cells (OPCs), because some exhibited the expression of glutathione S-transferase pi isoform in the nucleus. A recent publication showed that OPCs express PLP but not DM-20 mRNA. However, no OPCs were detected. We performed ISH with a cRNA probe that specifically recognizes PLP mRNA to successfully detect some OPCs. Additionally, OPCs were detected by ISH with a cRNA probe complementary to DM-20 mRNA that was digested via alkaline hydrolysis prior to ISH. These findings collectively demonstrate that PLP and DM-20 mRNA expression is restricted to oligodendrocyte-lineage cells, and imply that the undigested cRNA probe complementary to the full-length DM-20 mRNA sequence only recognizes DM-20 mRNA and not the PLP counterpart when applied to ISH without denaturation/digestion methods.

Published

2015

52. Induction of Schwann Cells from Rat Bone Marrow Mesenchymal Stem Cells

Author

Masaaki Kitada, Mari Dezawa, and Shohei Wakao

Subjects

Endothelial stem cell, Pathology, medicine.medical_specialty, medicine.anatomical_structure, Mesenchymal stem cell, medicine, Amniotic stem cells, Bone marrow, Rat Bone Marrow, Biology, Stem cell, Adult stem cell, Stem cell transplantation for articular cartilage repair

Published

2015

53. Choroid plexus ependymal cells host neural progenitor cells in the rat

Author

Akira Shimizu, Yutaka Itokazu, Akira Mizoguchi, Mari Dezawa, Chizuka Ide, Naoya Matsumoto, and Masaaki Kitada

Subjects

Ependymal Cell, Immunocytochemistry, Nerve Tissue Proteins, Biology, Mice, Cellular and Molecular Neuroscience, chemistry.chemical_compound, Microscopy, Electron, Transmission, Tubulin, Ependyma, Spheroids, Cellular, Precursor cell, Glial Fibrillary Acidic Protein, medicine, Animals, Rats, Wistar, Progenitor cell, Growth Substances, Cells, Cultured, Neurons, Mice, Inbred BALB C, Stem Cells, RNA-Binding Proteins, Cell Differentiation, Flow Cytometry, Antigens, Differentiation, Immunohistochemistry, Molecular biology, Neural stem cell, Rats, ErbB Receptors, medicine.anatomical_structure, Animals, Newborn, Neurology, chemistry, Choroid Plexus, Immunology, Neuroglia, Choroid plexus, Biomarkers, Bromodeoxyuridine

Abstract

We previously demonstrated that choroid plexus epithelial (modified ependymal) cells (CPECs) differentiated into astrocytes after grafting into the spinal cord. In the present study, we examined whether CPECs from rats at postnatal 1 day (P1), 7 day (P7), and 8 weeks (P8W) can function as neural progenitor cells that give rise to neurons and glial cells. Cell spheres were produced in cultures of whole tissue of the choroid plexus from the fourth ventricle of rats at each postnatal period. beta-tubulin class III (Tuj-1), glial fibrillary acid protein (GFAP)-, and O4-positive cells differentiated from cell spheres in the differentiation medium. We produced a monoclonal antibody 3E6 specifically labeling microvilli of CPECs. Using this monoclonal antibody, CPECs were isolated from the choroid plexus of P8W rats by cell sorter (FACS). Immunocytochemistry confirmed that there was no contamination from fibroblasts, endothelial cells, macrophages, or Schwann cells in the FACS-isolated 3E6-labeled cells. Cell spheres formed in the cultures of these 3E6-labeled CPECs. After expansion, these cell spheres gave rise to Tuj-1- (5%), GFAP- (45%), and O4-positive cells (0.16%). The remaining cells (45%) were unlabeled neural or glial markers. Some CPECs of the P8W rat were immunohistochemically stained with lineage-associated markers of Musashi-1 and epidermal growth factor-receptor (EGF-R). In addition, infusion of EGF or fibroblast growth factor-2 (FGF2) into the ventricle increased the number of bromodeoxyuridine (BrdU)-positive cells among CPECs from 0.03% (untreated) to 1.14% (38-fold, EGF) and 1.03% (35-fold, FGF2), respectively. These findings indicate that neural progenitor cells exist among CPECs in the rat.

Published

2005

54. Neurite outgrowth from hippocampal neurons is promoted by choroid plexus ependymal cells in vitro

Author

Masaaki Kitada, Akira Mizoguchi, Naoya Matsumoto, Chizuka Ide, and Kazushi Kimura

Subjects

Histology, Ependymal Cell, Neurite, Receptors, Nerve Growth Factor, Hippocampal formation, Biology, Hippocampus, Mice, Ependyma, Neurites, medicine, Animals, Cells, Cultured, Neurons, General Neuroscience, Cell Biology, Cadherins, Spinal cord, In vitro, Extracellular Matrix, Rats, Cell biology, medicine.anatomical_structure, Astrocytes, Culture Media, Conditioned, Choroid Plexus, Choroid plexus, Anatomy, Cell Adhesion Molecules, Neuroscience, Developmental biology, Astrocyte

Abstract

Choroid plexus ependymal cells (CPECs) were known to promote axonal growth when choroid plexus is grafted into the adult rat spinal cord. The present study was carried out to examine whether CPECs promote axonal outgrowth from neurons derived from the CNS in vitro. Hippocampal neurons were cocultured on CPEC monolayers. After 24 h, neurite extension was evaluated using various parameters in comparison with cultures grown on poly-L-lysine (PLL)-coated plates and cocultures grown on astrocyte monolayers. The primary neurite length and total neurite length were longest in the cocultures with CPECs. The number of primary neurites and the number of branches were larger in the cultures with CPECs than in the cultures on PLL-coated plates, but almost the same as in the cocultures with astrocytes. Next, we examined whether the neurite extension-promoting effect occurring within 24 h is due primarily to contact with the CPECs or to factors secreted by CPECs into the culture medium. The CPEC monolayers were killed by ethanol fixation, and neurons cultured on them. The neurons extended long neurites with elaborate branching, as in the case of cocultures grown on living CPECs. On the other hand, CPEC-conditioned medium exhibited less promoting effect on neurite outgrowth from hippocampal neurons. These results indicate that CPECs have a capacity to promote neurite outgrowth from CNS neurons in vitro , and that surface plasma membrane-bound components of CPECs strongly contribute to the enhancement of neurite outgrowth in the present coculture system.

Published

2004

55. Specific induction of neuronal cells from bone marrow stromal cells and application for autologous transplantation

Author

Mari Dezawa, Hiroshi Kanno, Mikio Hoshino, Hirotomi Cho, Naoya Matsumoto, Yutaka Itokazu, Nobuyoshi Tajima, Hitoshi Yamada, Hajime Sawada, Hiroto Ishikawa, Toshirou Mimura, Masaaki Kitada, Yoshihisa Suzuki, and Chizuka Ide

Subjects

Tyrosine 3-Monooxygenase, Cell Transplantation, Bone Marrow Cells, Transfection, Transplantation, Autologous, Article, Animals, Humans, Ciliary Neurotrophic Factor, Glial Cell Line-Derived Neurotrophic Factor, Nerve Growth Factors, Rats, Wistar, Cells, Cultured, Visual Cortex, Neurons, Receptors, Notch, Colforsin, Membrane Proteins, Parkinson Disease, General Medicine, Protein Structure, Tertiary, Rats, Phenotype, nervous system, Fibroblast Growth Factor 2, Stromal Cells, Biomarkers, Transcription Factors

Abstract

Bone marrow stromal cells (MSCs) have the capability under specific conditions of differentiating into various cell types such as osteocytes, chondrocytes, and adipocytes. Here we demonstrate a highly efficient and specific induction of cells with neuronal characteristics, without glial differentiation, from both rat and human MSCs using gene transfection with Notch intracellular domain (NICD) and subsequent treatment with bFGF, forskolin, and ciliary neurotrophic factor. MSCs expressed markers related to neural stem cells after transfection with NICD, and subsequent trophic factor administration induced neuronal cells. Some of them showed voltage-gated fast sodium and delayed rectifier potassium currents and action potentials compatible with characteristics of functional neurons. Further treatment of the induced neuronal cells with glial cell line–derived neurotrophic factor (GDNF) increased the proportion of tyrosine hydroxylase–positive and dopamine-producing cells. Transplantation of these GDNF-treated cells showed improvement in apomorphine-induced rotational behavior and adjusting step and paw-reaching tests following intrastriatal implantation in a 6-hydroxy dopamine rat model of Parkinson disease. This study shows that a population of neuronal cells can be specifically generated from MSCs and that induced cells may allow for a neuroreconstructive approach.

Published

2004

56. Alginate Enhances Elongation of Early Regenerating Axons in Spinal Cord of Young Rats

Author

Tadashi Hashimoto, Masayoshi Ohta, Kyoko Suzuki, Hirotomi Chou, Yoshihisa Suzuki, Masaaki Kitada, Sufan Wu, Chizuka Ide, Kazuya Kataoka, and Hongliang Bai

Subjects

Alginates, Biocompatible Materials, Lesion, Glucuronic Acid, medicine, Animals, Spinal Cord Injuries, Chemistry, Hexuronic Acids, Regeneration (biology), General Engineering, Anatomy, Spinal cord, Immunohistochemistry, Axons, Nerve Regeneration, Rats, Collagen gel, Microscopy, Electron, medicine.anatomical_structure, Spinal Cord, Regenerating axons, Collagen, medicine.symptom, Elongation, Astrocyte

Abstract

Freeze-dried alginate sponge cross-linked with covalent bonds has been demonstrated to enhance nerve regeneration in peripheral nerves and spinal cords. The present study examined, at early stages after surgery, the outgrowth of regenerating axons and reactions of astrocytes at the stump of transected spinal cord in young rats. Two segments (Th7-8) were resected, and alginate was implanted in the lesion. As controls, collagen gel was implanted in place of alginate or the lesion was left without implantation. Two and 4 weeks after surgery, nerve outgrowth and astrocyte reactions were examined. Many regenerating axons, some of which were accompanied by astrocytic processes, were found to extend from the stump into the alginate-implanted lesion. In the all nonimplanted animals, large cystic cavities were formed at both interfaces with no definite axonal outgrowth into the lesion. In collagen-implanted animals, cavity formation was found in some rats, and regenerating axons once formed at the stumps did not extend further into the lesion. Astrocytic processes extending into alginate-implanted lesion had no basal laminae, whereas those found in control experiments were covered by basal laminae. These findings suggest that alginate contributed to reducing the barrier composed of connective tissues and reactive astrocytic processes, and served as a scaffold for the outgrowth of regenerating axons and elongation of astrocytic processes.

Published

2004

57. Poly lactic acid-caprolactone copolymer tube with a denatured skeletal muscle segment inside as a guide for peripheral nerve regeneration: A morphological and electrophysiological evaluation of the regenerated nerves

Author

Nurru Mligiliche, Masaaki Kitada, Chizuka Ide, Katsuaki Endoh, Yasuhiko Tabata, Keiko Okamato, and Etsuko Fujimoto

Subjects

Sciatic Neuropathy, Polymers, Polyesters, Population, Nerve guidance conduit, Nerve fiber, Hindlimb, Nerve Fibers, Myelinated, Lactones, Absorbable Implants, medicine, Animals, Lactic Acid, Peripheral Nerves, Muscle, Skeletal, education, Caproates, Cell Size, education.field_of_study, Chemistry, Graft Survival, Skeletal muscle, General Medicine, Anatomy, Sciatic Nerve, Axons, Nerve Regeneration, Compound muscle action potential, Treatment Outcome, medicine.anatomical_structure, Tissue Transplantation, Rabbits, Sciatic nerve

Abstract

A biodegradable copolymer of poly L-lactic acid and epsilon-caprolactone (PLAC) was manufactured into a tube, in which a denatured skeletal muscle segment was placed longitudinally. This model tube was implanted as a guide to promote nerve regeneration across a 5 cm gap in the rabbit sciatic nerve. Five months after implantation, good nerve regeneration was found throughout the graft and in the distal host nerve. The population (29.6/16 x 10(2) microm(2)) of regenerated nerves in the graft was higher than that of the contralateral normal sciatic nerve (18.0/16 x 10(2) microm(2)). Regenerated nerve fibers extended to the distal host nerve. The number of myelinated fibers was 13.7/16 x 10(2) microm(2) at a level 1.5 cm from the distal suture. The diameters (below 2 microm) of most regenerated myelinated (nerves in the graft and in the distal host nerve were much smaller than those (6-8 microm) of normal nerves. Electrophysiological evaluation showed that the hindlimb muscle (gastrocnemius) was innervated by motor nerves in all animals 5 months after implantation. These results indicate that the PLAC tube with a denatured muscle segment inside provided good conditions for nerve fiber regrowth. The PLAC tube is thought to protect the denatured muscle segment from rapid dissociation in the host tissue.

Published

2003

58. Isolation of a set of genes expressed in the choroid plexus of the mouse using suppression subtractive hybridization

Author

Hitoshi Kitayama, Kazushi Kimura, Chizuka Ide, Naoya Matsumoto, Masaaki Kitada, and Makoto Noda

Subjects

Male, biology, General Neuroscience, Sequence Analysis, DNA, In situ hybridization, ABCA8, Molecular biology, Blot, Mice, Transthyretin, Suppression, Genetic, Cerebrospinal fluid, Gene Expression Regulation, Suppression subtractive hybridization, Choroid Plexus, biology.protein, Animals, Choroid plexus, sense organs, Gelsolin, In Situ Hybridization, Gene Library

Abstract

The choroid plexus produces cerebrospinal fluid, providing a specialized environment for the CNS. We previously demonstrated that choroid plexus ependymal cells can enhance nerve regeneration in vivo and promote neurite outgrowth in vitro. To understand the molecular mechanisms of choroid plexus functions, we isolated genes predominantly expressed in the mouse choroid plexus using suppression subtractive hybridization. Out of the 49 complementary DNA (cDNA) fragments isolated in two types of screening, 43 matched known sequences in the database and six were novel. In one type of screening where choroid plexus cDNAs were subtracted with cerebral cortex cDNAs, transthyretin and phosphodiesterase I alpha were predominant. This is consistent with previous reports and supports the authenticity of our approach. In the other type of screening, cDNAs derived from the choroid plexus of neonatal (postnatal day 5) mice were subtracted with cDNAs from the choroid plexus of adult mice. RNA blot and/or in situ hybridization confirmed abundant expression, in the mouse choroid plexus, of the mRNA encoding gelsolin, phospholipid transfer protein, ATP-binding cassette transporter A8 (ABCA8), androgen-inducible aldehyde reductase, and Na(+)/sulfate cotransporter SUT-1. Also, one novel gene (FS88) was found to be expressed in the choroid plexus from neonatal mice. Our data suggest that the choroid plexus cells produce molecules involved in processes such as prevention of fibrillization of amyloid beta-protein (transthyretin and gelsolin), lipid metabolism (phospholipid transfer protein and ABCA8), and detoxification (androgen-inducible aldehyde reductase).

Published

2003

59. Peripheral nerve regeneration through alginate gel: analysis of early outgrowth and late increase in diameter of regenerating axons

Author

Katsuaki Endo, Kyoko Suzuki, Masaaki Kitada, Tadashi Hashimoto, Sufan Wu, Yoshihiko Nishimura, Chizuka Ide, Kazuya Kataoka, and Yoshihisa Suzuki

Subjects

Male, Time Factors, Alginates, Schwann cell, Glucuronic Acid, Cell Movement, medicine, Animals, Peripheral Nerves, Rats, Wistar, Axon, Basement membrane, Chemistry, Hexuronic Acids, General Neuroscience, Regeneration (biology), Schwann cell migration, Anatomy, Axons, Nerve Regeneration, Rats, Cell biology, medicine.anatomical_structure, Peripheral nervous system, Neuroglia, Basal lamina, Gels

Abstract

Our previous study revealed that alginate gel cross-linked with covalent bonds promoted peripheral nerve regeneration in the cat and rat. The present study analyzed nerve regeneration through alginate gel in the early stages within 2 weeks and the late stages up to 21 months after implantation. Four days after surgery, regenerating axons grew without Schwann cell investment through the partially degraded alginate gel, being in direct contact with the alginate without a basal lamina covering. Numerous mast cells infiltrated into the alginate. One to 2 weeks after surgery, regenerating axons were surrounded by common Schwann cells to form small bundles, with some axons at the periphery being partly in direct contact with alginate. At the distal stump, numerous Schwann cells had migrated into the alginate 8-14 days after surgery. They had no basal laminae. The diameter of regenerated myelinated fibers was small (approximately 1 micro m) at 8 weeks, but increased in diameter, having a distribution pattern similar to that of normal nerve 21 months after surgery. Much better nerve regeneration was found in alginate gel-, than collagen sponge-, and fibrin glue-implanted distal stump 12 months after surgery. These results indicate that alginate gel has good biocompatibility for regenerating axon outgrowth and Schwann cell migration, and that regenerated fibers can have a diameter as thick as that of normal fibers in the long term. Alginate gel is a promising material for use as an implant for peripheral nerve regeneration.

Published

2002

60. New method for transplantation of neurosphere cells into injured spinal cord through cerebrospinal fluid in rat

Author

Kazuya Kataoka, Yoshihisa Suzuki, Sufan Wu, Chizuka Ide, Yoshihiko Nishimura, Miyako Kitaura, Hirotomi Chou, and Masaaki Kitada

Subjects

Pathology, medicine.medical_specialty, Green Fluorescent Proteins, Central nervous system, Biology, Fourth ventricle, Cisterna magna, Hippocampus, Subarachnoid Space, Animals, Genetically Modified, Rats, Sprague-Dawley, Fetus, Cerebrospinal fluid, Cell Movement, Tubulin, Neurosphere, Glial Fibrillary Acidic Protein, medicine, Animals, Brain Tissue Transplantation, Spinal cord injury, Spinal Cord Injuries, Cerebrospinal Fluid, Fourth Ventricle, General Neuroscience, Graft Survival, Recovery of Function, Anatomy, medicine.disease, Spinal cord, Immunohistochemistry, Nerve Regeneration, Rats, Transplantation, Luminescent Proteins, medicine.anatomical_structure, Pia Mater, Indicators and Reagents, Stem Cell Transplantation

Abstract

Here we report a novel method of supplying cultured neurosphere cells to the injured spinal cord, by injection of cells into the cerebrospinal fluid (CSF) through the fourth ventricle or cisterna magna. Hippocampus-derived neurosphere cells, isolated from a transgenic rat fetus expressing green fluorescent protein, were transplanted into the CSF of a rat with spinal cord injury. It was found that injected cells were extensively transported by CSF within the subarachnoidal space, and survived as clusters on the pial surface of the spinal cord. The most notable finding was that a large number of injected cells migrated into the lesion site and integrated into the injured spinal cord tissues.

Published

2002

61. Migration, integration, and differentiation of hippocampus-derived neurosphere cells after transplantation into injured rat spinal cord

Author

Yoshihiko Nishimura, Kazuya Kataoka, Masaaki Kitada, Yoshihisa Suzuki, Chizuka Ide, Miyako Kitaura, Jun Takahashi, and Sufan Wu

Subjects

Pathology, medicine.medical_specialty, Alginates, Green Fluorescent Proteins, Central nervous system, Biology, Hippocampus, Animals, Genetically Modified, Rats, Sprague-Dawley, Cell Movement, Tubulin, Neurosphere, Glial Fibrillary Acidic Protein, medicine, Animals, Brain Tissue Transplantation, Cells, Cultured, Spinal Cord Injuries, Spinal Cord Regeneration, Glial fibrillary acidic protein, Stem Cells, General Neuroscience, Graft Survival, Cell Differentiation, Anatomy, Spinal cord, Immunohistochemistry, Neural stem cell, Rats, Transplantation, Luminescent Proteins, medicine.anatomical_structure, Spinal Cord, biology.protein, Indicators and Reagents, Stem cell, Stem Cell Transplantation

Abstract

Hippocampus-derived neurospheres were prepared from transgenic rat fetuses expressing green fluorescent protein (GFP), and transplanted into an alginate-filled lesion of young rat spinal cord. One, two and four weeks after transplantation, a large number of grafted cells survived, many of which expressed immunoreactivity for glial fibrillary acidic protein, and a few expressed immunoreactivity for beta-tubulin III. The grafted cells closely attached to the host tissue including astrocytes at the border of the lesion. It was notable that numerous GFP-positive cells had migrated within host spinal cord tissue up to 2 mm away from the implanted site 4 weeks postoperation. These results demonstrate that rat fetal hippocampus-derived neurosphere cells could survive, differentiate, extensively migrate, and integrate well into the host spinal cord tissue.

Published

2001

62. [Untitled]

Author

Chizuka Ide, Masanori Taketomi, Naoya Matsumoto, Shushovan Chakrabortty, Kazushi Kimura, and Masaaki Kitada

Subjects

Histology, Ependymal Cell, Neurite, General Neuroscience, Cell Biology, Anatomy, Biology, Fourth ventricle, In vitro, Cell biology, medicine.anatomical_structure, Dorsal root ganglion, medicine, Choroid plexus, Growth cone, Astrocyte

Abstract

The epithelial cells of the choroid plexus are a continuation of the ventricular ependymal cells and are regarded as modified ependymal cells. The present study was carried out to determine the influence of choroid plexus ependymal cells (CPECs) on axonal growth in vitro. Choroid plexuses were dissected from the fourth ventricle of postnatal day-1–10 mice, mechanically dissociated, and plated in fibronectin-coated culture dishes. CPECs had spread into monolayers with few endothelial cells in 3-week cultures. Some macrophages were scattered on the monolayer of CPECs. Dorsal root ganglia (DRG) were excised from mouse fetuses of 14-day gestation, dissociated with trypsin and cocultured on the CPEC monolayers. For comparison, dissociated DRG neurons were cocultured on astrocyte monolayers or cultured on laminin-coated plates. After 4.5 h culturing, the cultures were fixed and immunohistochemically double-stained for neurites and CPECs using antibodies against β-tubulin III and S-100 β, respectively. It was demonstrated that neurons extended many long neurites with elaborate branching on the surface of S-100-stained CPECs. In contrast, DRG neurons cultured on the astrocytes and on the laminin-coated plates had much shorter primary neurites with fewer branches than those cultured on the CPECs. The total length of neurites including primary neurites and their branches, of a single DRG neuron was 285 ± 14, 395 ± 15 and 565 ± 12 μm on the laminin-coated plates, on astrocytes and on CPECs, respectively. Scanning electron microscopy revealed extension of neurites with well-developed growth cones on the ependymal cells. These results suggest that CPECs have a great capacity to promote neurite outgrowth from DRG neurons in vitro.

Published

2000

63. Distribution of synaptosomal-associated protein 25 in nerve growth cones and reduction of neurite outgrowth by botulinum neurotoxin A without altering growth cone morphology in dorsal root ganglion neurons and PC-12 cells

Author

S Kozaki, Akira Mizoguchi, Yasusuke Hirasawa, S Kawano, Masaaki Kitada, T Ohmukai, Masahide Takahashi, Mikihiro Shirasu, Seiichiro Okajima, T Morihara, Chizuka Ide, T Tsujihara, Kazuo Tamai, and Kazushi Kimura

Subjects

Vesicle fusion, Synaptosomal-Associated Protein 25, Neurite, Immunoelectron microscopy, Mice, Inbred Strains, Nerve Tissue Proteins, Biology, PC12 Cells, Mice, Dorsal root ganglion, Ganglia, Spinal, Neurites, medicine, Animals, Neurotoxin, Syntaxin, Botulinum Toxins, Type A, Microscopy, Immunoelectron, Growth cone, Neurons, General Neuroscience, Membrane Proteins, Axons, Rats, Cell biology, medicine.anatomical_structure, Biochemistry, sense organs

Abstract

Synaptosomal-associated protein 25 has been regarded as one of the target-associated soluble N-ethylmaleimide-sensitive fusion attachment protein receptors essential for exocytosis of vesicles in synapses. We have previously reported that cleavage of syntaxin, which is another target-associated soluble N-ethylmaleimide-sensitive fusion attachment protein receptor, with botulinum neurotoxin C1 resulted in inhibition of neurite extension and morphological changes including growth cone collapse and large vacuole formation. As an attempt to explore the mechanism of growth cone extension, we examined the ultrastructural localization of synaptosomal-associated protein 25 in growth cones with or without treatment of botulinum neurotoxin A, which cleaves synaptosomal-associated protein 25. In dorsal root ganglion neurons, light microscopy demonstrated synaptosomal-associated protein 25 immunoreactivity throughout the neurons, including the cell bodies, neurites and growth cones. Using electron microscopy, gold signals immunoreactive for synaptosomal-associated protein 25 were identified diffusely in the cytoplasm of the growth cones. In contrast, in PC-12 cells, a large number of gold signals were localized on the plasma membranes. High levels of signal were also found in the cytoplasm in the central region of the growth cones. We also confirmed that botulinum neurotoxin A treatment reduced neurite extension by about 50%. However, both in dorsal root ganglion neurons and in PC-12 cells we found no differences in the ultrastructure nor in the localization of synaptosomal-associated protein 25 between growth cones with and without toxin treatment. These results indicate that cleavage of synaptosomal-associated protein 25 inhibits growth cone extension in a manner different than that of syntaxin cleavage. The results of this study suggest the possibility that synaptosomal-associated protein 25 is involved in growth cone extension through a process independent of vesicle fusion.

Published

1999

64. Abstracts

Author

Mamoru Nagano, Atuko Fujioka, Koh Shinoda, Maki YOSHIDA, Mayumi NISHI, Zenro KIZAKI, Tadashi SAWADA, Mitsuhiro KAWATA, Kiyoshi KUROKAWA, Maki MURATA, Hisao YAMADA, Motoi KUDO, Nobuteru USUDA, Keiju KAMIJO, Ayami NAKAZAWA, Naoko OGIWARA, Masashi YAMADA, Kohei JOHKURA, Johbu ITOH, Kenji KAWAI, Akihiko SEARIZAWA, Kazuhiko YASUMURA, Kenji OGAWA, R. Yoshiyuki OSAMURA, Yawara SUMI, Masanori T. ITOH, Minoru YOSHIDA, Sadaki Yokota, Akira Sawaguchi, Jun-ichi Kawano, Ryoko Nagaike, Tsutomu Oinuma, Tatsuo Suganuma, Tsuyoshi IWATA, Hitoshi OZAWA, Emi INUI, Osamu UKIMURA, Munekado KOJIMA, Tsuneharu MIKI, Tomomi YAMAMOTO, Yasuaki SHIBATA, Masashi SHIN, Yoshitaka HISHIKAWA, Akira YAMAGUCHI, Toshimitsu KOBAYASHI, Takehiko KOJI, Norifumi FUTAGAWA, Hiroshi TAKANO, Tetsuji NAGATA, Kizashi NAGATA, Shigeru TAKETANI, Masasuke ARAKI, M. Araki, Y. Isobe, Y. Nakane, M. Tudsuki, Nobuaki SHIKATA, Airo TSUBURA, Nobukazu ARAKI, Teruhiko Okada, Vadim S. Zinchuk, Toshihiro Kobayashi, Harumichi Seguchi, Yuko Ito, Yoshinori Otsuki, Xin Li, Yutaka Yatomi, Yoshie Miura, Ryohei Katoh, Yukio Ozaki, Akira Kawaoi, Takao SENDA, Mayumi Matsuta, Morimasa Matsuta, Toshihide Akasaka, Hidehiko Suzuki, Naoya Yamazaki, Kazuhiro Yagila, Hitoshi Okamura, Akiko Ogawa, Katutosi Ito, Masako Maeda, Hirokazu Ohtaki, Hisayuki Funahashi, Seiji Shioda, Mayuko Ikebe, Hiroaki Matsumoto, Katsutoshi Ito, TOMOYUKI MATSUDA, KENSHI KAKIHARA, MASASHI UEDA, YOSHITAKA TAMADA, SEIJI HAYASHI, NORIO IIJIMA, MASAKI TANAKA, YASUHIKO IBATA, H. NAGATA, S. TAKEKOSHI, T. OHNISHI, J. ITOH, H. HASEGAWA, Y. YAMAMOTO, S. OHNO, K. WATANABE, Y Kataoka, N Iijima, K Kakihara, Y Tamada, S Hayashi, M Tanaka, S Hinuma, H Matsumoto, C Kitada, H Onda, H Honjo, Y Ibata, Keisuke INOUE, Yoshitaka TAMADA, Norio IIJIMA, Seiji HAYASHI, Masaki TANAKA, Akihiko ISHIHARA, Yasuhiko IBATA, Ikuko NAGATSU, Nobuyuki KARASAWA, Keiki YAMADA, Mikihiro Shirasu, Kazushi Kimura, Akira Mizoguchi, Chizuka Ide, Naoya Matsumoto, Masaaki Kitada, Shushovan Chakrabortty, Hideho Ueda, Takeshi Baba, Yasuko Kato, Ichiro Takayama, Yasuhisa Fujii, Nobuo Terada, and Shinichi Ohno

Subjects

Histology, Physiology, Cell Biology, Biochemistry, Pathology and Forensic Medicine

Published

1999

65. Transplantation of Bone Marrow Stromal Cell-Derived Neural Precursor Cells Ameliorates Deficits in a Rat Model of Complete Spinal Cord Transection

Author

Takahiro Morita, Akira Sumiyoshi, Toshiki Endo, Jorge J. Riera, Shohei Wakao, Masaaki Kitada, Yasumasa Kuroda, Misaki Aizawa-Kohama, Dai Matsuse, Mari Dezawa, Teiji Tominaga, and Ryuta Kawashima

Subjects

Biomedical Engineering, lcsh:Medicine, Random Allocation, Neurosphere, Medicine, Premovement neuronal activity, Animals, Rats, Wistar, Spinal cord injury, Spinal Cord Injuries, Bone Marrow Transplantation, Neurons, Transplantation, biology, business.industry, lcsh:R, Cell Differentiation, Cell Biology, Recovery of Function, Spinal cord, medicine.disease, Magnetic Resonance Imaging, Neural stem cell, Nerve Regeneration, Rats, Disease Models, Animal, medicine.anatomical_structure, nervous system, Synaptophysin, biology.protein, Female, Bone marrow, Stromal Cells, business, Neuroscience, Stem Cell Transplantation

Abstract

After severe spinal cord injury, spontaneous functional recovery is limited. Numerous studies have demonstrated cell transplantation as a reliable therapeutic approach. However, it remains unknown whether grafted neuronal cells could replace lost neurons and reconstruct neuronal networks in the injured spinal cord. To address this issue, we transplanted bone marrow stromal cell-derived neural progenitor cells (BM-NPCs) in a rat model of complete spinal cord transection 9 days after the injury. BM-NPCs were induced from bone marrow stromal cells (BMSCs) by gene transfer of the Notch-1 intracellular domain followed by culturing in the neurosphere method. As reported previously, BM-NPCs differentiated into neuronal cells in a highly selective manner in vitro. We assessed hind limb movements of the animals weekly for 7 weeks to monitor functional recovery after local injection of BM-NPCs to the transected site. To test the sensory recovery, we performed functional magnetic resonance imaging (fMRI) using electrical stimulation of the hind limbs. In the injured spinal cord, transplanted BM-NPCs were confirmed to express neuronal markers 7 weeks following the transplantation. Grafted cells successfully extended neurites beyond the transected portion of the spinal cord. Adjacent localization of synaptophysin and PSD-95 in the transplanted cells suggested synaptic formations. These results indicated survival and successful differentiation of BM-NPCs in the severely injured spinal cord. Importantly, rats that received BM-NPCs demonstrated significant motor recovery when compared to the vehicle injection group. Volumes of the fMRI signals in somatosensory cortex were larger in the BM-NPC-grafted animals. However, neuronal activity was diverse and not confined to the original hind limb territory in the somatosensory cortex. Therefore, reconstruction of neuronal networks was not clearly confirmed. Our results indicated BM-NPCs as an effective method to deliver neuronal lineage cells in a severely injured spinal cord. However, reestablishment of neuronal networks in completed transected spinal cord was still a challenging task.

Published

2013

66. Isolation, culture and evaluation of multilineage-differentiating stress-enduring (Muse) cells

Author

Toru Murakami, Shohei Wakao, Masaaki Kitada, Yasumasa Kuroda, Mari Dezawa, and Makoto Nojima

Subjects

Muse cell, Stage-Specific Embryonic Antigens, Cellular differentiation, Induced Pluripotent Stem Cells, Cell Culture Techniques, Bone Marrow Cells, Receptors, Cell Surface, Biology, General Biochemistry, Genetics and Molecular Biology, Mesoderm, Antigens, CD, Humans, Antigens, Tumor-Associated, Carbohydrate, Cell Lineage, Cell potency, Cells, Cultured, Stem cell transplantation for articular cartilage repair, Stem Cells, Endoglin, Amniotic stem cells, Cell Differentiation, Flow Cytometry, Embryonic stem cell, Cell biology, Immunology, Stem cell, Adult stem cell

Abstract

Multilineage-differentiating stress-enduring (Muse) cells are distinct stem cells in mesenchymal cell populations with the capacity to self-renew, to differentiate into cells representative of all three germ layers from a single cell, and to repair damaged tissues by spontaneous differentiation into tissue-specific cells without forming teratomas. We describe step-by-step procedures for isolating and evaluating these cells. Muse cells are also a practical cell source for human induced pluripotent stem (iPS) cells with markedly high generation efficiency. They can be collected as cells that are double positive for stage-specific embryonic antigen-3 (SSEA-3) and CD105 from commercially available mesenchymal cells, such as adult human bone marrow stromal cells and dermal fibroblasts, or from fresh adult human bone marrow samples. Under both spontaneous and induced differentiation conditions, they show triploblastic differentiation. It takes 4–6 h to collect and 2 weeks to confirm the differentiation and self-renewal capacity of Muse cells.

Published

2013

67. Displacement of Acid Phosphatase and Alkaline Phosphatase Proteins in the Rat Kidney during a Dehydration Procedure. An Advantage of Ultrathin Frozen Sections for Detecting Precise Localization of an Enzyme Activity

Author

Masakazu Miyamura, Hiroshi Yamashita, Koji Kishimoto, Osamu Fukushima, Takafumi Yatsu, Masaaki Kitada, and Hideki Arakawa

Subjects

Frozen section procedure, Histology, biology, Physiology, Chemistry, Acid phosphatase, Rat kidney, Cell Biology, Biochemistry, Enzyme assay, Pathology and Forensic Medicine, Dehydration Procedure, biology.protein, Alkaline phosphatase, Displacement (orthopedic surgery)

Published

1995

68. The elite and stochastic model for iPS cell generation: multilineage-differentiating stress enduring (Muse) cells are readily reprogrammable into iPS cells

Author

Masaaki Kitada, Mari Dezawa, and Shohei Wakao

Subjects

Pluripotent Stem Cells, education.field_of_study, Histology, Models, Statistical, Mechanism (biology), Stochastic modelling, Computer science, Mesenchymal stem cell, Population, Cell Differentiation, Mesenchymal Stem Cells, Cell Biology, Fibroblasts, Pathology and Forensic Medicine, Humans, education, Induced pluripotent stem cell, Neuroscience, Adult stem cell, Cell Proliferation

Abstract

Induced pluripotent stem (iPS) cells have attracted a great deal of attention, although the mechanism by which they are generated is still not fully understood. Currently, two theories, the stochastic and elite models, have been proposed. Some reports provide theoretical support for the stochastic model. Other reports, however, support the elite model. For example, some human fibroblasts, such as Multilineage-differentiating stress enduring (Muse) cells, are reported to be pluripotent and a primary source of iPS cells. Thus, the mechanism of iPS cell generation continues to be debated. In this review, we discuss the properties of the original cell source, such as the components of the original populations and the potential of each population to become iPS cells, and further discuss the implications of the two theories for iPS cell research. © 2012 International Society for Advancement of Cytometry

Published

2012

69. Morphologic and gene expression criteria for identifying human induced pluripotent stem cells

Author

Toru Murakami, Mari Dezawa, Yasumasa Kuroda, Akira Niwa, Masaaki Kitada, Shohei Wakao, and Fumitaka Ogura

Subjects

Homeobox protein NANOG, Cytoplasm, Somatic cell, Cellular differentiation, Green Fluorescent Proteins, Induced Pluripotent Stem Cells, Cell Culture Techniques, Gene Expression, lcsh:Medicine, Biology, Polymerase Chain Reaction, Molecular Genetics, Kruppel-Like Factor 4, Mice, SOX2, Molecular Cell Biology, Genetics, Animals, Humans, CDX2 Transcription Factor, Induced pluripotent stem cell, lcsh:Science, Embryonic Stem Cells, Cell Nucleus, Homeodomain Proteins, Multidisciplinary, Gene Expression Profiling, SOXB1 Transcription Factors, Stem Cells, lcsh:R, Computational Biology, Mesenchymal Stem Cells, Transfection, Fibroblasts, Molecular biology, Embryonic stem cell, Adult Stem Cells, Retroviridae, Gene Expression Regulation, embryonic structures, RNA, lcsh:Q, Stem cell, Cell Nucleolus, Research Article, Developmental Biology

Abstract

Induced pluripotent stem (iPS) cells can be generated from somatic cells by the forced expression of four factors, Oct3/4, Sox2, Klf4, and c-Myc. While a great variety of colonies grow during induction, only a few of them develop into iPS cells. Researchers currently use visual observation to identify iPS cells and select colonies resembling embryonic stem (ES) cells, and there are no established objective criteria. Therefore, we exhaustively analyzed the morphology and gene expression of all the colonies generated from human fibroblasts after transfection with four retroviral vectors encoding individual factors (192 and 203 colonies in two experiments) and with a single polycistronic retroviral vector encoding all four factors (199 and 192 colonies in two experiments). Here we demonstrate that the morphologic features of emerged colonies can be categorized based on six parameters, and all generated colonies that could be passaged were classified into seven subtypes in colonies transfected with four retroviral vectors and six subtypes with a single polycistronic retroviral vector, both including iPS cell colonies. The essential qualifications for iPS cells were: cells with a single nucleolus; nucleus to nucleolus (N/Nls) ratio ∼2.19: cell size ∼43.5 µm(2): a nucleus to cytoplasm (N/C) ratio ∼0.87: cell density in a colony ∼5900 cells/mm(2): and number of cell layer single. Most importantly, gene expression analysis revealed for the first time that endogenous Sox2 and Cdx2 were expressed specifically in iPS cells, whereas Oct3/4 and Nanog, popularly used markers for identifying iPS cells, are expressed in colonies other than iPS cells, suggesting that Sox2 and Cdx2 are reliable markers for identifying iPS cells. Our findings indicate that morphologic parameters and the expression of endogenous Sox2 and Cdx2 can be used to accurately identify iPS cells.

Published

2012

70. Isolation of adult human pluripotent stem cells from mesenchymal cell populations and their application to liver damages

Author

Shohei, Wakao, Masaaki, Kitada, Yasumasa, Kuroda, and Mari, Dezawa

Subjects

Adult, Pluripotent Stem Cells, Stage-Specific Embryonic Antigens, Reverse Transcriptase Polymerase Chain Reaction, Lentivirus, Cell Differentiation, Mesenchymal Stem Cells, Cell Separation, Flow Cytometry, Immunohistochemistry, End Stage Liver Disease, HEK293 Cells, Humans, Antigens, Tumor-Associated, Carbohydrate, Stem Cell Transplantation

Abstract

We have found a novel type of pluripotent stem cells, Multilineage-differentiating stress enduring (Muse) cells that can be isolated from mesenchymal cell populations. Muse cells are characterized by stress tolerance, expression of pluripotency markers, self-renewal, and the ability to differentiate into endodermal-, mesodermal-, and ectodermal-lineage cells from a single cell, demonstrating that they are pluripotent stem cells. They can be isolated as cells positive for stage-specific embryonic antigen-3, a human pluripotent stem cell marker. Here, we introduce the isolation method for Muse cells and the effect of transplantation of these cells on chronic liver diseases.

Published

2011

71. Isolation of Adult Human Pluripotent Stem Cells from Mesenchymal Cell Populations and Their Application to Liver Damages

Author

Yasumasa Kuroda, Masaaki Kitada, Mari Dezawa, and Shohei Wakao

Subjects

Transplantation, Mesenchymal stem cell, HEK 293 cells, Stem cell, Biology, Induced pluripotent stem cell, Embryonic stem cell, Adult stem cell, Stem cell transplantation for articular cartilage repair, Cell biology

Abstract

We have found a novel type of pluripotent stem cells, Multilineage-differentiating stress enduring (Muse) cells that can be isolated from mesenchymal cell populations. Muse cells are characterized by stress tolerance, expression of pluripotency markers, self-renewal, and the ability to differentiate into endodermal-, mesodermal-, and ectodermal-lineage cells from a single cell, demonstrating that they are pluripotent stem cells. They can be isolated as cells positive for stage-specific embryonic antigen-3, a human pluripotent stem cell marker. Here, we introduce the isolation method for Muse cells and the effect of transplantation of these cells on chronic liver diseases.

Published

2011

72. Human umbilical cord-derived mesenchymal stromal cells differentiate into functional Schwann cells that sustain peripheral nerve regeneration

Author

Shohei Wakao, Misaki Kohama, Hidenori Akutsu, Tatsutoshi Nakahata, Yoshinori Fujiyoshi, Mari Dezawa, Masaaki Kitada, Toshio Heike, Hideki Makinoshima, Jun Ichi Kira, Dai Matsuse, Hideo Harigae, Akihiro Umezawa, and Kouki Nishikawa

Subjects

Adult, Male, Stromal cell, Immunoelectron microscopy, Schwann cell, Tretinoin, Biology, Pathology and Forensic Medicine, Umbilical Cord, Cellular and Molecular Neuroscience, Myelin, medicine, Animals, Humans, Peripheral Nerves, Axon, Rats, Wistar, integumentary system, Mesenchymal stem cell, Cell Differentiation, Mesenchymal Stem Cells, General Medicine, Recovery of Function, Sciatic Nerve, Axons, Cell biology, Nerve Regeneration, Rats, medicine.anatomical_structure, nervous system, Neurology, Peripheral nerve injury, Neuroglia, Intercellular Signaling Peptides and Proteins, Neurology (clinical), Schwann Cells, Stromal Cells, tissues, Neuroscience, Biomarkers, Stem Cell Transplantation

Abstract

Human umbilical cord-derived mesenchymal stromal cells (UC-MSCs) that are available from cell banks can be induced to differentiate into various cell types, thereby making them practical potential sources for cell-based therapies. In injured peripheral nerves, Schwann cells (SCs) contribute to functional recovery by supporting axonal regeneration and myelin reconstruction. Here, we first demonstrate a system to induce UC-MSCs to differentiate into cells with SC properties (UC-SCs) by treatment with β-mercaptoethanol followed by retinoic acid and a set of specific cytokines. The UC-SCs are morphologically similar to SCs and express SC markers, including P0, as assessed by immunocytochemistry and reverse transcription polymerase chain reaction. Transplantation of UC-SCs into transected sciatic nerves in adult rats enhanced nerve regeneration. The effectiveness of UC-SCs for axonal regeneration was comparable to that of authentic human SCs based on histological criteria and functional recovery. Immunohistochemistry and immunoelectron microscopy also demonstrated myelination of regenerated axons by UC-SCs. These findings indicate that cells with SC properties and with the ability to support axonal regeneration and reconstruct myelin can be successfully induced from UC-MSCs to promote functional recovery after peripheral nerve injury. This system may be applicable for the development of cell-based therapies.

Published

2010

73. Lectins as a tool for detecting neural stem/progenitor cells in the adult mouse brain

Author

Yasumasa Kuroda, Masaaki Kitada, and Mari Dezawa

Subjects

Peanut agglutinin, Male, Histology, Wheat Germ Agglutinins, Subventricular zone, Mice, Agglutinin, Neural Stem Cells, Neurosphere, Lectins, medicine, Animals, Phytohemagglutinins, Ecology, Evolution, Behavior and Systematics, biology, Histocytochemistry, Neurogenesis, Lectin, Brain, Flow Cytometry, Neural stem cell, Wheat germ agglutinin, Cell biology, Mice, Inbred C57BL, medicine.anatomical_structure, nervous system, Biochemistry, biology.protein, Anatomy, Plant Lectins, Biotechnology

Abstract

Glycoconjugates are biopolymers that are broadly distributed in the central nervous system, including the cell surface of neural stem cells or neural precursor cells (NSCs/NPCs). Glycoconjugates can be recognized by carbohydrate-binding proteins, lectins. Two lectins, Phaseolus vulgaris lectin agglutinin E-form (PHA-E4) and wheat germ agglutinin (WGA) have been reported to be useful in isolating NSCs/NPCs by fluorescence-activated cell sorting (FACS) or immunopanning methods. In this study, we analyzed the lectin-binding properties of NSCs/NPCs in two neurogenic regions of the adult mouse brain to determine whether PHA-E4 and WGA exhibit specific binding patterns on sections and whether there are other lectins presenting the binding pattern similar to those of PHA-E4 and WGA in lectin histochemistry. Among nine types of lectins, peanut agglutinin was localized to the white matter and four lectins bound to cells within the subventricular zone (SVZ) of the lateral ventricle. Lectin histochemistry combined with immunohistochemistry demonstrated that one lectin, Ricinus communis agglutinin, specifically detected type A neuronal precursors and that the remaining three lectins, Agaricus bisporus agglutinin (ABA), PHA-E4, and WGA, recognized type B NSCs and type C transient amplifying cells in the SVZ. These three lectins also recognized type 1 quiescent neural progenitors and type 2a amplifying neural progenitors in the subgranular layer of the dentate gyrus. Lectin histochemistry of the neurosphere culture also yielded similar results. These observations suggest that, in addition to PHA-E4 and WGA, ABA lectin may also be applicable in FACS or immunopanning for the isolation of NSCs/NPCs.

Published

2010

74. Long-term observation of auto-cell transplantation in non-human primate reveals safety and efficiency of bone marrow stromal cell-derived Schwann cells in peripheral nerve regeneration

Author

Yutaka Itokazu, Noboru Teramoto, Takuya Hayashi, Mari Dezawa, Tomoaki Takamoto, Takayuki Ose, Kazuhiro Koshino, Masaaki Kitada, Dai Matsue, Shohei Wakao, Hiroshi Watabe, Hidehiro Iida, Misaki Kohama, and Yasuhiko Tabata

Subjects

Male, Pathology, medicine.medical_specialty, Stromal cell, Time Factors, Median Neuropathy, Neural Conduction, Schwann cell, Bone Marrow Cells, Biology, Transplantation, Autologous, Cell therapy, Myelin, Peripheral nerve, Developmental Neuroscience, Fluorodeoxyglucose F18, medicine, Animals, Cells, Cultured, Bone Marrow Transplantation, Motor Neurons, Transdifferentiation, Mesenchymal stem cell, Cell Differentiation, Recovery of Function, Nerve injury, Median Nerve, Nerve Regeneration, Transplantation, Monkey, Disease Models, Animal, Macaca fascicularis, medicine.anatomical_structure, Neurology, Motor Skills, Peripheral nervous system, Positron-Emission Tomography, Mesenchymal stem cells, Schwann Cells, medicine.symptom, Stromal Cells, Cell Division

Abstract

Based on their differentiation ability, bone marrow stromal cells (MSCs) are a good source for cell therapy. Using a cynomolgus monkey peripheral nervous system injury model, we examined the safety and efficacy of Schwann cells induced from MSCs as a source for auto-cell transplantation therapy in nerve injury. Serial treatment of monkey MSCs with reducing agents and cytokines induced their differentiation into cells with Schwann cell properties at a very high ratio. Expression of Schwann cell markers was confirmed by both immunocytochemistry and reverse transcription-polymerase chain reaction. Induced Schwann cells were used for auto-cell transplantation into the median nerve and followed-up for 1 year. No abnormalities were observed in general conditions. Ki67-immunostaining revealed no sign of massive proliferation inside the grafted tube. Furthermore, 18F-fluorodeoxygluocose-positron emission tomography scanning demonstrated no abnormal accumulation of radioactivity except in regions with expected physiologic accumulation. Restoration of the transplanted nerve was corroborated by behavior analysis, electrophysiology and histological evaluation. Our results suggest that auto-cell transplantation therapy using MSC-derived Schwann cells is safe and effective for accelerating the regeneration of transected axons and for functional recovery of injured nerves. The practical advantages of MSCs are expected to make this system applicable for spinal cord injury and other neurotrauma or myelin disorders where the acceleration of regeneration is expected to enhance functional recovery.

Published

2009

75. Induction system of neural and muscle lineage cells from bone marrow stromal cells; a new strategy for tissue reconstruction in degenerative diseases

Author

Masaaki, Kitada and Mari, Dezawa

Subjects

Neurons, Muscle Cells, Dopamine, Bone Marrow Cells, Cell Differentiation, Mesenchymal Stem Cells, Neurodegenerative Diseases, Mesenchymal Stem Cell Transplantation, Muscular Disorders, Atrophic, Nerve Regeneration, Stroke, Parkinsonian Disorders, Animals, Humans, Spinal Cord Injuries

Abstract

Since bone marrow stromal cells (MSCs) are easily accessible both from healthy donors and patients, and can be expanded on a therapeutic scale, they have attracted attention for cell-based therapy. MSCs contribute to the protection of host tissue after transplantation by Immune modulation and trophic effect. They also have an ability to differentiate into other cell kinds that will replenish lost cells in the degenerated tissue. This review discusses the potential of MSCs for tissue reconstruction in neuro- and muscle-degenerative diseases and their differentiation capacity into functional cells.

Published

2009

76. Practical induction system for dopamine-producing cells from bone marrow stromal cells using spermine-pullulan-mediated reverse transfection method

Author

Yasuhiko Tabata, Masaaki Kitada, Mari Dezawa, Kentaro Nagane, and Shohei Wakao

Subjects

Programmed cell death, Stromal cell, Cell Survival, Dopamine, Cell, Biomedical Engineering, Intracellular Space, Bioengineering, Bone Marrow Cells, Biology, Gene delivery, Transfection, Biochemistry, Regenerative medicine, Biomaterials, Mice, Species Specificity, medicine, Animals, Humans, Transgenes, Luciferases, Cell Shape, Glucans, Neurons, Microscopy, Confocal, Tyrosine hydroxylase, DNA, Molecular biology, medicine.anatomical_structure, Macaca, Spermine, Bone marrow, Stromal Cells, Reverse transfection, Plasmids

Abstract

Introduction of various kinds of exogenous genes is an important step for control of differentiation in stem cell biology and regenerative medicine. However, some kinds of cells are vulnerable to manipulations such as gene delivery. In this context, a gene introduction method with higher efficiency and safety is required. Bone marrow stromal cells (BMSCs) offer possibilities for clinical application because of their potential for expandability and ability to be auto-transplanted. In this study, we established an efficient induction system of dopamine-producing neuronal cells from BMSCs in several species using the spermine-pullulan-mediated reverse transfection technique. In this system, introduced exogenous plasmid genes were successfully transcribed and expressed as proteins in the cytoplasm of BMSCs with the smallest number of cell death. Microtubule-associated protein 2 and anti-beta-tubulin class III+ neurons were successfully delivered from human, monkey, and mouse BMSCs, and further treatment with trophic factors promoted differentiation of induced neuronal cells into dopamine-producing cells that were positive for tyrosine hydroxylase and secreted dopamine after high K+ stimulation in high-performance liquid chromatography analysis. Our study indicates the availability of the reverse transfection method for the induction of dopamine-producing neuronal cells from BMSCs, which is expected to apply to cell-based therapy in Parkinson's disease.

Published

2009

77. Induction system of neural and muscle lineage cells from bone marrow stromal cells; a new strategy for tissue reconstruction in degenerative diseases

Author

Masaaki Kitada and Dezawa, M.

Subjects

Parkinson's disease, Spinal cord injury (SCI), 576 - Biología celular y subcelular. Citología

Abstract

Since bone marrow stromal cells (MSCs) are easily accessible both from healthy donors and patients, and can be expanded on a therapeutic scale, they have attracted attention for cell-based therapy. MSCs contribute to the protection of host tissue after transplantation by Immune modulation and trophic effect. They also have an ability to differentiate into other cell kinds that will replenish lost cells in the degenerated tissue. This review discusses the potential of MSCs for tissue reconstruction in neuro- and muscledegenerative diseases and their differentiation capacity into functional cells.

Published

2009

78. A new monoclonal antibody, A3B10, specific for astrocyte-lineage cells recognizes calmodulin-regulated spectrin-associated protein 1 (Camsap1)

Author

Hiroaki Asou, Toshiyuki Ueki, Masahiro Yamamoto, Atsushi Ishige, Kazunori Yoshimura, Masaaki Kitada, Chika Seiwa, Kenji Watanabe, Yasushi Shimoda, and Jin Nakahara

Subjects

Male, Blotting, Western, Molecular Sequence Data, Nerve Tissue Proteins, Biology, Cellular and Molecular Neuroscience, Mice, Neurosphere, Glial Fibrillary Acidic Protein, medicine, Animals, Cell Lineage, Amino Acid Sequence, Rats, Wistar, Microscopy, Immunoelectron, Mice, Knockout, Mice, Inbred BALB C, Glial fibrillary acidic protein, Stem Cells, Neurogenesis, Antibodies, Monoclonal, Brain, GFAP stain, Molecular biology, Immunohistochemistry, Neural stem cell, Rats, Neuroepithelial cell, Cytoskeletal Proteins, medicine.anatomical_structure, Astrocytes, biology.protein, Female, Antibody, Microtubule-Associated Proteins, Biomarkers, Astrocyte

Abstract

Recent studies of adult neurogenesis of the mammalian central nervous system have suggested unexpected plasticity and complexity of neural cell ontogenesis. Redefinition and reconstitution of cell classification and lineage relationships, especially between glial and neural precursors, are an urgent and crucial concern. In the present study, we describe a new monoclonal antibody, A3B10, which was produced by immunizing mice with the membrane fraction prepared from astrocyte-enriched primary neural cell cultures. Immunohistochemistry of brain sections, including brains from glial fibrillary acidic protein (GFAP)-deficient mice and primary mixed neural cell cultures, as well as immunoblot analysis and immunoelectron microscopy, have revealed that 1) A3B10 recognizes a majority of cells in ependyma in neonatal and adult rats, 2) A3B10 stains almost all GFAP+ cells and some S100β+ cells in the corpus callosum, 3) A3B10 specifically stains astrocytes in vitro in primary cultures of rat embryonic cerebral hemispheres, 4) A3B10 equally stains ependymal cells of wild-type and GFAP-deficient mice, and 5) A3B10 antigen might construct intermediate filament bundles with GFAP and/or vimentin. These data suggested that the antibody labels a wide array of astorcytic-lineage cells including astrocytes, astrocyte precursors, and neural stem cells. Screening a cDNA library derived from rat embryonic brain has revealed that the antibody recognizes calmodulin-regulated spectrin-associated protein 1 (Camsap1). Thus this antibody may provide not only a new marker to identify astrocyte-lineage cells but also a new target molecule to elucidate the ontogeny, development, and pathophysiological functions of astrocyte-lineage cells. © 2008 Wiley-Liss, Inc.

Published

2008

79. [Neural repair]

Author

Masaaki, Kitada and Mari, Dezawa

Subjects

Neurons, Cytological Techniques, Cell- and Tissue-Based Therapy, Animals, Humans, Bone Marrow Cells, Cell Differentiation, Mesenchymal Stem Cells, Neurodegenerative Diseases, Schwann Cells, Regenerative Medicine, Spinal Cord Injuries

Abstract

Recent progress of stem cell biology gives us the hope for neural repair. We have established methods to specifically induce functional Schwann cells and neurons from bone marrow stromal cells (MSCs). The effectiveness of these induced cells was evaluated by grafting them either into peripheral nerve injury, spinal cord injury, or Parkinson' s disease animal models. MSCs-derived Schwann cells supported axonal regeneration and re-constructed myelin to facilitate the functional recovery in peripheral and spinal cord injury. MSCs-derived dopaminergic neurons integrated into host striatum and contributed to behavioral repair. In this review, we introduce the differentiation potential of MSCs and finally discuss about their benefits and drawbacks of these induction systems for cell-based therapy in neuro-traumatic and neuro-degenerative diseases.

Published

2008

80. Development of NG2 neural progenitor cells requires Olig gene function

Author

Santosh Kesari, Keith L. Ligon, David H. Rowitch, David J. Anderson, Masaaki Kitada, Heather A. Arnett, Tao Sun, Charles D. Stiles, and John A. Alberta

Subjects

Mice, Transgenic, Nerve Tissue Proteins, Biology, OLIG2, Mice, medicine, Basic Helix-Loop-Helix Transcription Factors, Animals, Humans, Cell Lineage, Progenitor cell, Antigens, Transcription factor, Neurons, Multidisciplinary, Stem Cells, Brain, Oligodendrocyte Transcription Factor 2, Biological Sciences, Embryo, Mammalian, Embryonic stem cell, Oligodendrocyte, Neural stem cell, Cell biology, Mice, Inbred C57BL, Oligodendroglia, medicine.anatomical_structure, Spinal Cord, nervous system, CSPG4, Immunology, Proteoglycans, Stem cell, Caltech Library Services

Abstract

In the adult central nervous system, two distinct populations of glial cells expressing the chondroitin sulfate proteoglycan NG2 have been described: bipolar progenitor cells and more differentiated “synantocytes.” These cells have diverse neurological functions, including critical roles in synaptic transmission, repair, and regeneration. Despite their potential importance, the genetic factors that regulate NG2 cell development are poorly understood, and the relationship of synantocytes to the oligodendroglial lineage, in particular, remains controversial. Here, we show that >90% of embryonic and adult NG2 cells express Olig2, a basic helix–loop–helix transcription factor required for oligodendrocyte lineage specification. Analysis of mice lacking Olig function demonstrates a failure of NG2 cell development at embryonic and perinatal stages that can be rescued by addition of a transgene containing the human OLIG2 locus. These findings show a general requirement for Olig function in NG2 cell development and highlight further roles for Olig transcription factors in neural progenitor cells.

Published

2006

81. Transcription factor co-expression patterns indicate heterogeneity of oligodendroglial subpopulations in adult spinal cord

Author

Masaaki Kitada and David H. Rowitch

Subjects

Male, Oligodendrocyte Transcription Factor 2, Central nervous system, Autophagy-Related Proteins, Cell Count, Nerve Tissue Proteins, Biology, SOXE Transcription Factors, OLIG2, White matter, Cellular and Molecular Neuroscience, Mice, medicine, Basic Helix-Loop-Helix Transcription Factors, Animals, Cell Lineage, Antigens, Myelin Sheath, Cell Proliferation, Homeodomain Proteins, Stem Cells, High Mobility Group Proteins, Intracellular Signaling Peptides and Proteins, Gene Expression Regulation, Developmental, Cell Differentiation, Zebrafish Proteins, Immunohistochemistry, Neural stem cell, Oligodendrocyte, Mice, Inbred C57BL, Oligodendroglia, medicine.anatomical_structure, Homeobox Protein Nkx-2.2, Neurology, Spinal Cord, Neuroglia, Proteoglycans, Neuroscience, Transcription Factors

Abstract

Oligodendrocytes and their precursors serve critical roles in the maintenance of neurological function. Although activity of the transcription factors (TFs) Olig1, Olig2, Sox10, and Nkx2.2 is required during early oligodendrocyte development, their later expression in adult central nervous system is rather poorly characterized. Here we have analyzed co-expression patterns of these transcriptional proteins in the mouse cervical spinal cord. Our findings indicate that TF co-expression patterns describe heterogeneity in adult oligodendroglial populations (1) in distinct sub-regions of grey and white matter and (2) with respect to level of maturation from proliferating precursors to myelinating oligodendrocytes. Our findings suggest that TF co-expression patterns identify and might regulate distinct functional classes of grey and white matter oligodendroglia.

Published

2006

82. Evidence for motoneuron lineage-specific regulation of Olig2 in the vertebrate neural tube

Author

Dong In Yuk, Sovann Kaing, Brian P. Hafler, Keith L. Ligon, Charles D. Stiles, Tao Sun, Masaaki Kitada, David H. Rowitch, and Hans R. Widlund

Subjects

Motor neuron, Chromosomes, Artificial, Bacterial, Bacterial Artificial Chromosome (BAC), Lineage mapping, cis-regulation, Mice, Transgenic, Nerve Tissue Proteins, Biology, Neural tube, OLIG2, 03 medical and health sciences, Mice, 0302 clinical medicine, Neuroblast, medicine, Transcriptional regulation, Basic Helix-Loop-Helix Transcription Factors, Animals, Humans, Cell Lineage, Enhancer, Molecular Biology, Transcription factor, 030304 developmental biology, Mice, Knockout, Motor Neurons, 0303 health sciences, Stem Cells, Cell Differentiation, Cell Biology, Oligodendrocyte Transcription Factor 2, Oligodendrocyte, Molecular biology, Cell biology, Oligodendroglia, medicine.anatomical_structure, Enhancer Elements, Genetic, Spinal Cord, Olig2, 030217 neurology & neurosurgery, Developmental Biology

Abstract

Within the motoneuron precursor (pMN) domain of the developing spinal cord, the bHLH transcription factor, Olig2, plays critical roles in pattern formation and the generation of motor neuron and oligodendrocyte precursors. How are the multiple functions of Olig2 regulated? We have isolated a large BAC clone encompassing the human OLIG2 locus that rescues motor neuron and oligodendrocyte development but not normal pattern formation in Olig2−/− embryos. Within the BAC clone, we identified a conserved 3.6 kb enhancer sub-region that directs reporter expression specifically in the motor neuron lineage but not oligodendrocyte lineage in vivo. Our findings indicate complex regulation of Olig2 by stage- and lineage-specific regulatory elements. They further suggest that transcriptional regulation of Olig2 is involved in segregation of pMN neuroblasts.

Published

2005

83. Increase in bFGF-responsive neural progenitor population following contusion injury of the adult rodent spinal cord

Author

Masahiro Yamaguchi, Chizuka Ide, Mari Dezawa, Yi Xu, and Masaaki Kitada

Subjects

Green Fluorescent Proteins, Mice, Transgenic, Nerve Tissue Proteins, Biology, Glial scar, Nestin, Rats, Sprague-Dawley, Mice, Intermediate Filament Proteins, Neurosphere, medicine, Animals, Progenitor cell, Promoter Regions, Genetic, Spinal cord injury, Spinal Cord Injuries, Cell Proliferation, Neurons, General Neuroscience, Multipotent Stem Cells, Stem Cells, medicine.disease, Spinal cord, Immunohistochemistry, Radial glial cell, Neural stem cell, Cell biology, Rats, medicine.anatomical_structure, Immunology, Fibroblast Growth Factor 2

Abstract

The number of neural progenitor cells, especially nestin+ cells or BrdU-uptake cells is sparse in the normal adult rodent spinal cord. However, in the present study, we show that after spinal cord injury (SCI), many ordinarily quiescent cells were activated to become nestin+ and undergo mitosis (BrdU+) in the ependymal layer as well as in the parenchyma of the spinal cord. Nestin+ cells and BrdU+ cells were in most cases immunohistochemically GFAP+, some of which displayed radial glial cell morphology and partly participated in the border formation of the lesion. The culturing of injured rat spinal cord tissues generated more neurospheres earlier than did the culturing of intact tissues, and these neurosphere cells were multipotent and bFGF-responsive. Immunohistochemical analysis showed that there existed many bFGF+ cells after SCI, the number of which were almost 15 times greater than that in an intact spinal cord. Increased bFGF production after SCI might activate quiescent progenitor cells, and thus initiate their cell proliferation. Finally, SCI to the nestin-promoter green fluorescent protein (GFP) transgenic mice showed broad proliferation of progenitor cells that were induced in the injured spinal cord. The culturing of injured spinal cord tissues from these transgenic mice provides direct evidence that neurospheres can be generated by SCI-activated nestin+ cells. Thus, the activation of bFGF-responsive progenitor cells and the concomitant increase in the population of bFGF+ cells following SCI might be beneficial for spinal cord repair if these progenitor cells are properly manipulated.

Published

2005

84. Grafting of the Choroid Plexus

Author

Shushovan Chakrabortty, Yutaka Itokazu, Naoya Matsumoto, Masaaki Kitada, Kazushi Kimura, and Chizuka Ide

Subjects

Pathology, medicine.medical_specialty, Grafting (decision trees), medicine, Choroid plexus, Biology

Published

2005

85. Implantation of neural stem cells via cerebrospinal fluid into the injured root

Author

Yoshihisa Suzuki, Mari Dezawa, Masayoshi Ohta, Namiko Ishikawa, Toru Noda, Chizuka Ide, Masaaki Kitada, Naoya Matsumoto, Kazuya Kataoka, Hirotomi Chou, and Shigehiko Suzuki

Subjects

Nerve guidance conduit, Schwann cell, Biology, Subarachnoid Space, Animals, Genetically Modified, Rats, Sprague-Dawley, Fetus, medicine, Animals, Peripheral Nerves, Axon, Radiculopathy, Cells, Cultured, Cerebrospinal Fluid, Injections, Intraventricular, Neurons, Fourth Ventricle, General Neuroscience, Stem Cells, Graft Survival, Cell Differentiation, Neural stem cell, Axons, Cell biology, Nerve Regeneration, Rats, Neuroepithelial cell, Disease Models, Animal, medicine.anatomical_structure, Treatment Outcome, nervous system, Astrocytes, Neuroglia, Schwann Cells, Stem cell, Spinal Nerve Roots, Neuroscience, Adult stem cell, Stem Cell Transplantation

Abstract

In avulsion injury of the dorsal root, regenerating axons cannot extend through the entry zone, i.e. the transition zone between peripheral and central nervous systems, due to the discontinuity between Schwann cells and astrocytes. We infused neural stem cells through the 4th ventricle in an attempt to enhance axonal growth in injured dorsal roots. Infused stem cells were attached to, and integrated into, the lesion of the root and became associated with axons in the same manner as Schwann cells or perineurial sheath cells in the peripheral nerve, and as astrocytes in the central nerve area. These findings suggest that neural stem cells integrated by infusion through CSF might have a beneficial effect on nerve regeneration by inducing a continuity of Schwann cells and astrocytes at the transition zone.

Published

2004

86. In vitro and in vivo characterization of pigment epithelial cells differentiated from primate embryonic stem cells

Author

Yoshiki Sasai, Masaaki Kitada, Sotaro Ooto, Hiroshi Kawasaki, Masatoshi Haruta, Hirofumi Suemori, Norio Nakatsuji, Yoshihito Honda, Chizuka Ide, Masayo Takahashi, and Kaori Amemiya

Subjects

Retinal degeneration, cis-trans-Isomerases, Stromal cell, Cell Survival, Cellular differentiation, Blotting, Western, Biology, C-Mer Tyrosine Kinase, Rats, Mutant Strains, chemistry.chemical_compound, fluids and secretions, Phagocytosis, Proto-Oncogene Proteins, medicine, Animals, Eye Proteins, Fluorescent Antibody Technique, Indirect, Pigment Epithelium of Eye, Cells, Cultured, c-Mer Tyrosine Kinase, Reverse Transcriptase Polymerase Chain Reaction, Stem Cells, Retinal Degeneration, Membrane Proteins, Proteins, Receptor Protein-Tyrosine Kinases, Retinal, Cell Differentiation, biochemical phenomena, metabolism, and nutrition, medicine.disease, Phosphoproteins, Embryonic stem cell, eye diseases, Coculture Techniques, Cell biology, Rats, Macaca fascicularis, chemistry, RPE65, Zonula Occludens-1 Protein, sense organs, Stem cell, Carrier Proteins, Biomarkers, Photoreceptor Cells, Vertebrate, Stem Cell Transplantation

Abstract

Purpose To determine whether primate embryonic stem (ES) cell-derived pigment epithelial cells (ESPEs) have the properties and functions of retinal pigment epithelial (RPE) cells in vitro and in vivo. Methods Cynomolgus monkey ES cells were induced to differentiate into pigment epithelial cells by coculturing them with PA6 stromal cells in a differentiating medium. The expanded, single-layer ESPEs were examined by light and electron microscopy. The expression of standard RPE markers by the ESPEs was determined by RT-PCR, Western blot, and immunocytochemical analyses. The ESPEs were transplanted into the subretinal space of 4-week-old Royal College of Surgeons (RCS) rats, and the eyes were analyzed immunohistochemically at 8 weeks after grafting. The effect of the ESPE graft on the visual function of RCS rats was estimated by optokinetic reflex. Results The expanded ESPEs were hexagonal and contained significant amounts of pigment. The ESPEs expressed typical RPE markers: ZO-1, RPE65, CRALBP, and Mertk. They had extensive microvilli and were able to phagocytose latex beads. When transplanted into the subretinal space of RCS rats, the grafted ESPEs enhanced the survival of the host photoreceptors. The effects of the transplanted ESPEs were confirmed by histologic analyses and behavioral tests. Conclusions The ESPEs had morphologic and physiological properties of normal RPE cells, and these findings suggest that these cells may provide an unlimited source of primate cells to be used for the study of pathogenesis, drug development, and cell-replacement therapy in eyes with retinal degenerative diseases due to primary RPE dysfunction.

Published

2004

87. Dissemination and proliferation of neural stem cells on the spinal cord by injection into the fourth ventricle of the rat: a method for cell transplantation

Author

Chizuka Ide, Hongliang Bai, Yoshihisa Suzuki, Sufan Wu, Kazuya Kataoka, Masayoshi Ohta, Toru Noda, Hirotomi Chou, and Masaaki Kitada

Subjects

Biology, Fourth ventricle, Hippocampus, Animals, Genetically Modified, Rats, Sprague-Dawley, Neurosphere, medicine, Animals, Cells, Cultured, Injections, Intraventricular, Neurons, Fourth Ventricle, Pia mater, General Neuroscience, Stem Cells, Cell Differentiation, Anatomy, Spinal cord, Neural stem cell, Cord lining, Rats, Transplantation, medicine.anatomical_structure, Spinal Cord, Adult stem cell, Stem Cell Transplantation

Abstract

We examined the distribution of hippocampus-derived neural stem cells on the spinal cord surface for up to 3 weeks following injection through the fourth ventricle. The injected cells were disseminated as tiny spots on the pia mater of the spinal cord and proliferated into large cell-clusters. On both the dorsal and ventral side, cell clusters increased in number rapidly up to 5 days after injection and thereafter decreased gradually due to the coalition of neighbouring clusters. Concomitantly, individual cell clusters continuously increased in size, occupying almost 50% of the spinal cord surface. Cell attachment was usually found around blood vessels, along which cells invaded into the spinal cord. In the injured site, cells migrated into the lesion and were integrated into the spinal cord tissue, some of which had differentiated into astrocytes 1-2 weeks after injection. BrdU-uptake experiments demonstrated that the transplanted cells proliferated within the host cerebrospinal fluid. These results indicate that application of neural stem cells through the ventricle is an effective method to disseminate cells all over the spinal cord and that they can migrate and be integrated into the injured spinal cord.

Published

2003

88. Bone marrow stromal cells enhance differentiation of cocultured neurosphere cells and promote regeneration of injured spinal cord

Author

Yoko Ejiri, Toru Noda, Chizuka Ide, Masayoshi Ohta, Masaaki Kitada, Hirotomi Chou, Sufan Wu, Kazuya Kataoka, Yoshihisa Suzuki, and Hongliang Bai

Subjects

Male, Stromal cell, Cell Count, Animals, Genetically Modified, Rats, Sprague-Dawley, Cellular and Molecular Neuroscience, Fetus, Neurosphere, Medicine, Animals, Microscopy, Immunoelectron, Spinal cord injury, Cells, Cultured, Spinal Cord Injuries, Bone Marrow Transplantation, Microscopy, Confocal, business.industry, Regeneration (biology), Mesenchymal stem cell, Cell Differentiation, Recovery of Function, Spinal cord, medicine.disease, Immunohistochemistry, Coculture Techniques, Cell biology, Nerve Regeneration, Rats, Transplantation, medicine.anatomical_structure, Spinal Cord, Immunology, Bone marrow, Stromal Cells, business

Abstract

Transplantation of bone marrow stromal cells (MSCs) has been regarded as a potential approach for promoting nerve regeneration. In the present study, we investigated the influence of MSCs on spinal cord neurosphere cells in vitro and on the regeneration of injured spinal cord in vivo by grafting. MSCs from adult rats were cocultured with fetal spinal cord-derived neurosphere cells by either cell mixing or making monolayered-feeder cultures. In the mixed cell cultures, neuroshpere cells were stimulated to develop extensive processes. In the monolayered-feeder cultures, numerous processes from neurosphere cells appeared to be attracted to MSCs. In an in vivo experiment, grafted MSCs promoted the regeneration of injured spinal cord by enhancing tissue repair of the lesion, leaving apparently smaller cavities than in controls. Although the number of grafted MSCs gradually decreased, some treated animals showed remarkable functional recovery. These results suggest that MSCs might have profound effects on the differentiation of neurosphere cells and be able to promote regeneration of the spinal cord by means of grafting.

Published

2003

89. Comparison of the axonal and glial reactions between the caudal and rostral border in the cryoinjured dorsal funiculus of the rat spinal cord

Author

Masaaki, Kitada, Akira, Mizoguchi, Koujiro, Tohyama, Akinori, Ohtsubo, Etsuko, Fujimoto, Shushovan, Chakrabortty, and Chizuka, Ide

Abstract

Axonal and glial reactions to traumatic injury were compared between the caudal and rostral border of the lesion after freeze-injury to the C3 dorsal funiculus by attaching a liquid nitrogen-cooled copper probe to the dorsum of the rat spinal cord. The axonal and glial changes were examined up to 60 days postoperative by light and electron microscopy and immunohistochemistry for neurofilaments. Regenerative axonal changes and the appearance of numerous undifferentiated cells were found at the caudal border 7 days after cryoinjury. In contrast, such axonal and cellular reactions were scarce at the rostral border. Undifferentiated cells clearly manifested their phenotypes by differentiating into oligodendrocytes or astrocytes 11 days postinjury. The results indicated that glial cell reactions occurred in association with regenerative axonal changes at the proximal stump of the injured nerve fibers, suggesting that regenerating and demyelinated naked axons could be responsible for the appearance of the immature glial cells.

Published

2003

90. Nogo-A expression in mature oligodendrocytes of rat spinal cord in association with specific molecules

Author

Chizuka Ide, Nagatoki Kinoshita, Masanori Taketomi, Toru Noda, Masaaki Kitada, Kazushi Kimura, Hiroaki Asou, and Takashi Nakamura

Subjects

Male, Cytoplasm, Neurite, Nogo Proteins, Central nervous system, Myelin, Compact myelin, Tubulin, mental disorders, medicine, Animals, Rats, Wistar, Myelin Sheath, biology, General Neuroscience, Myelin Basic Protein, Oligodendrocyte, Myelin basic protein, Cell biology, Rats, Oligodendroglia, medicine.anatomical_structure, Animals, Newborn, Spinal Cord, COS Cells, biology.protein, Neuroglia, Neuroscience, psychological phenomena and processes, Myelin Proteins

Abstract

Nogo-A is known as an oligodendrocyte/myelin-associated molecule having an inhibitory effect on neurite outgrowth in the central nervous system. During development, starting from P21 Nogo-A was detected in the cytoplasm of mature oligodendrocytes with compact myelin sheaths in the rat spinal cord. COS7 cells transfected with recNogo-A displayed strong Nogo-A immunoreactivity in their cytoplasm as well as on the mitotic spindle. Nogo-A was not detected in membrane protein fractions from transfected plus biotinylated COS7 cells. Nogo-A was co-immunoprecipitated with alpha-tubulin and myelin basic protein (MBP) from rat brain tissue. These results show that Nogo-A is expressed in association with tubulin and MBP in the mature oligodendrocytes.

Published

2002

91. Immunohistochemical and electron microscopic study of invasion and differentiation in spinal cord lesion of neural stem cells grafted through cerebrospinal fluid in rat

Author

Yoshihisa Suzuki, Yoshihiko Nishimura, Sufan Wu, Kazuya Kataoka, Toru Noda, Hongliang Bai, Masaaki Kitada, and Chizuka Ide

Subjects

Pathology, medicine.medical_specialty, Immunoelectron microscopy, Cellular differentiation, Green Fluorescent Proteins, Biology, Hippocampus, Animals, Genetically Modified, Immunoenzyme Techniques, Rats, Sprague-Dawley, Cellular and Molecular Neuroscience, Fetal Tissue Transplantation, Pregnancy, Neurosphere, medicine, Animals, Brain Tissue Transplantation, Microscopy, Immunoelectron, Cells, Cultured, Cerebrospinal Fluid, Injections, Intraventricular, Neurons, Fourth Ventricle, Stem Cells, Cell Differentiation, Anatomy, Spinal cord, Immunohistochemistry, Neural stem cell, Rats, Neuroepithelial cell, Luminescent Proteins, Oligodendroglia, medicine.anatomical_structure, Spinal Cord, Astrocytes, Female, Indicators and Reagents, Schwann Cells, Stem cell, Spinal Nerve Roots, Adult stem cell, Stem Cell Transplantation

Abstract

Neurospheres were obtained by culturing hippocampal cells from transgenic rat fetuses (E16) expressing green fluorescent protein (GFP). The neurosphere cells were injected into the cerebrospinal fluid (CSF) through the 4th ventricle of young rats (4 weeks old) that had been given a contusion injury at T8-9 of the spinal cord. The injected neural stem cells were transported through the CSF to the spinal cord, attached to the pial surface at the lesion, and invaded extensively into the spinal cord tissue as well as into the nerve roots. The grafted stem cells survived well in the host spinal cord for as long as 8 months after transplantation. Immunohistochemical study showed that many grafted stem cells had differentiated into astrocytes at 1-4 months, and some into oligodendrocytes at 8 months postoperatively. Immunoelectron microscopy showed that the grafted stem cells were well integrated into the host tissue, extending their processes around nerve fibers in the same manner as astrocytes. In addition, grafted stem cells within nerve roots closely surrounded myelinated fibers or were integrated into unmyelinated fiber bundles; those associated with myelinated fibers formed basal laminae on their free surface, whereas those associated with unmyelinated fibers were directly attached to axons and Schwann cells, indicating that grafted stem cells behaved like Schwann cells in the nerve roots.

Published

2002

92. Correction for Kuroda et al., Unique multipotent cells in adult human mesenchymal cell populations

Author

Taeko Shigemoto, Yoshinori Fujiyoshi, Hideki Makinoshima, Yukihiro Tanimura, Ayumu Inutsuka, Masaaki Kitada, Hideo Akashi, Tatsutoshi Nakahata, Yasumasa Kuroda, Mari Dezawa, Yo-ichi Nabeshima, Kouki Nishikawa, Akira Niwa, Makoto Goda, Yoko Nabeshima, and Shohei Wakao

Subjects

Multidisciplinary, Mesenchymal stem cell, Cancer research, Biology, Corrections

Published

2014

93. Grafting of detergent-denatured skeletal muscles provides effective conduits for extension of regenerating axons in the rat sciatic nerve

Author

Masaaki Kitada, Chizuka Ide, and Nurru Mligiliche

Subjects

Histology, Neurofilament, Materials science, Detergents, Transplantation, Autologous, Basement Membrane, chemistry.chemical_compound, Type IV collagen, Basal (phylogenetics), Laminin, medicine, Animals, Sodium dodecyl sulfate, Rats, Wistar, Muscle, Skeletal, Microscopy, Confocal, biology, Sodium Dodecyl Sulfate, Anatomy, Immunohistochemistry, Sciatic Nerve, Axons, Nerve Regeneration, Rats, Microscopy, Electron, Biological detergent, medicine.anatomical_structure, chemistry, biology.protein, Basal lamina, Sciatic nerve

Abstract

The basal laminae of muscle fibers, when treated by denaturing methods including freeze thawing, have been used as conduits for regenerating nerves. In this study, we developed a new method for denaturing skeletal muscle fibers through treatment with a biological detergent, sodium dodecyl sulfate. Laminin and type IV collagen proteins of muscle fiber basal laminae were preserved after the detergent treatment. A segment of detergent-denatured muscle was grafted to a 1-cm defect of the rat sciatic nerve. One week after grafting, regenerating axons immunostained for neurofilaments were seen extending within laminin-positive muscle fiber basal lamina tubes. Four weeks after grafting, numerous myelinated axons at a much higher level than the control unoperated sciatic nerve, were found in the middle of the graft. They were smaller in diameter than those in the control nerve. Distal host nerves were well reinnervated 4 weeks after grafting. These findings suggest that the basal laminae of detergent-denatured muscle fibers provide effective conduits for regenerating axons.

Published

2001

94. Alginate, a bioresorbable material derived from brown seaweed, enhances elongation of amputated axons of spinal cord in infant rats

Author

Katsuaki Endo, Yoshihiko Nishimura, Kyoko Suzuki, Katsunori Ohnishi, Masaaki Kitada, Masao Tanihara, Kazuya Kataoka, Yoshihisa Suzuki, and Chizuka Ide

Subjects

Male, Alginates, Central nervous system, Biomedical Engineering, Biotin, Phaeophyta, Horseradish peroxidase, Biomaterials, medicine, Animals, Axon, Rats, Wistar, Spinal Cord Regeneration, Horseradish Peroxidase, Spinal Cord Injuries, biology, Electromyography, Regeneration (biology), Anatomy, Prostheses and Implants, Spinal cord, Immunohistochemistry, Axons, Rats, Electrophysiology, Microscopy, Electron, medicine.anatomical_structure, Cross-Linking Reagents, Freeze Drying, Gliosis, Animals, Newborn, Spinal Cord, biology.protein, Female, medicine.symptom, Locomotion, Astrocyte

Abstract

Freeze-dried alginate sponge crosslinked with covalent bonds was developed in our laboratory and has been demonstrated to enhance peripheral nerve regeneration. In this study, we examined spinal cord repair using alginate sponge in infant rats. On postnatal day 8-12, the spinal cord was transversely resected at Th7-Th8 to produce a 2-mm gap. The gap was filled with alginate sponge in the alginate group. For the control group, the gap was left empty. In the alginate group, the recovery of evoked electromyogram and sensory-evoked potentials 6 weeks after surgery indicated that elongation of axons could establish electrophysiologically functional projections through the gap. A histological study revealed that myelinated and unmyelinated axons, surrounded by a perineurial-like structure, had elongated across the gap. An immunohistochemical examination revealed that elongation of astrocytic processes and/or migration of astrocytes into the alginate sponge was induced, whereas astrocyte gliosis was reduced at the interface between the implanted alginate and the host spinal cord, compared with the control group. However, a horseradish peroxidase tracing study revealed ascending and descending fibers had also elongated into the gap and reentered the other stump of the transected spinal cord beyond the gap. These results suggest that alginate might provide a permissive microenvironment for elongation of spinal cord axons.

Published

2001

95. Grafting of choroid plexus ependymal cells promotes the growth of regenerating axons in the dorsal funiculus of rat spinal cord: a preliminary report

Author

Yoshihisa Suzuki, Masanori Taketomi, Shushovan Chakrabortty, T. Akira Mizoguchi, Saburo Kawaguchi, Chizuka Ide, Naoya Matsumoto, T. Katsuaki Endoh, Masaaki Kitada, and Soki Kikukawa

Subjects

Male, Ependymal Cell, Calcitonin Gene-Related Peptide, Central nervous system, Biology, Fourth ventricle, Developmental Neuroscience, Ependyma, medicine, Animals, Brain Tissue Transplantation, Axon, Rats, Wistar, Horseradish Peroxidase, Spinal Cord Injuries, Fluorescent Dyes, Graft Survival, Anatomy, Spinal cord, Immunohistochemistry, Sciatic Nerve, Axons, Nerve Regeneration, Rats, Posterior Horn Cells, Disease Models, Animal, medicine.anatomical_structure, nervous system, Neurology, Spinal nerve, Choroid Plexus, Choroid plexus, Female, Sciatic nerve

Abstract

Nerve regeneration in the central nervous system has been studied by grafting various tissues and cells. In the present study, we demonstrated that choroid plexus ependymal cells can promote nerve regeneration when grafted into spinal cord lesions. The choroid plexus was excised from the fourth ventricle of adult rats (Wistar), minced into small fragments, and grafted into the dorsal funiculus at the C2 level in adult rat spinal cord from the same strain. Electron microscopy and fluorescence histochemistry showed that ependymal cells of the grafted choroid plexus intimately interacted with growing axons, serving to support the massive growth of regenerating axons. CGRP-positive fibers closely interacted with grafted ependymal cells. HRP injection at the sciatic nerve showed that numerous HRP-labeled regenerating fibers from the fasciculus gracilis extended into the graft 7 days after grafting. This regenerating axons from the fasciculus gracilis was maintained for at least 10 months, with some axons elongating rostrally into the dorsal funiculus. Evoked potentials of long duration were recorded at a level ca. 5 mm rostral to the lesion in the rats 8 to 10 months after grafting. These findings indicate that choroid plexus ependymal cells have the ability to facilitate axonal growth in vivo, suggesting that they may be a promising candidate as graft for the promotion of nerve regeneration in the spinal cord.

Published

2001

96. Exploring the glial progenitor cells in the intact adult spinal cord

Author

Mari Dezawa, Yutaka Itokazu, Chizuka Ide, and Masaaki Kitada

Subjects

Pathology, medicine.medical_specialty, medicine.anatomical_structure, General Neuroscience, medicine, General Medicine, Progenitor cell, Biology, Spinal cord

Published

2007

97. 1108 Expressions of integrin alpha 6 subunit during mouse siatic nerve development

Author

Takuya, Hayakashi, primary, Masaaki, Kitada, additional, and Chizuka, Ide, additional

Published

1997

98. Axonal regeneration in the central nervous system is enhanced by ependymal cell transplants

Author

Akira Mizoguchi, Masaaki Kitada, Shushovan Chakrabortty, and Chizuka Ide

Subjects

medicine.anatomical_structure, Ependymal Cell, General Neuroscience, Regeneration (biology), Central nervous system, medicine, General Medicine, Biology, Cell biology

Published

1998

99. Neurite outgrowth from hippocampal neurons is promoted by choroid plexus ependymal cells in vitro.

Author

Kazushi Kimura, Naoya Matsumoto, Masaaki Kitada, Akira Mizoguchi, and Chizuka Ide

Abstract

Choroid plexus ependymal cells (CPECs) were known to promote axonal growth when choroid plexus is grafted into the adult rat spinal cord. The present study was carried out to examine whether CPECs promote axonal outgrowth from neurons derived from the CNS in vitro. Hippocampal neurons were cocultured on CPEC monolayers. After 24 h, neurite extension was evaluated using various parameters in comparison with cultures grown on poly-L-lysine (PLL)-coated plates and cocultures grown on astrocyte monolayers. The primary neurite length and total neurite length were longest in the cocultures with CPECs. The number of primary neurites and the number of branches were larger in the cultures with CPECs than in the cultures on PLL-coated plates, but almost the same as in the cocultures with astrocytes. Next, we examined whether the neurite extension-promoting effect occurring within 24 h is due primarily to contact with the CPECs or to factors secreted by CPECs into the culture medium. The CPEC monolayers were killed by ethanol fixation, and neurons cultured on them. The neurons extended long neurites with elaborate branching, as in the case of cocultures grown on living CPECs. On the other hand, CPEC-conditioned medium exhibited less promoting effect on neurite outgrowth from hippocampal neurons. These results indicate that CPECs have a capacity to promote neurite outgrowth from CNS neurons in vitro, and that surface plasma membrane-bound components of CPECs strongly contribute to the enhancement of neurite outgrowth in the present coculture system. [ABSTRACT FROM AUTHOR]

Published

2004

100. Alginate Enhances Elongation of Early Regenerating Axons in Spinal Cord of Young Rats.

Author

Kazuya Kataoka, Yoshihisa Suzuki, Masaaki Kitada, Tadashi Hashimoto, Hirotomi Chou, Hongliang Bai, Masayoshi Ohta, Sufan Wu, Kyoko Suzuki, and Chizuka Ide

Published

2004