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4. Проблема изотопного состава железа Земли и Луны. Измерения δ 57 Fe в образцах лунного грунта “Луна”-16-20-24 (доклад на ХХII-ом симпозиуме по геохимии стабильных изотопов, Москва, 29–31 октября 2019)

Author

Галимов, Э. М., primary, Okabayashi, S., additional, Yokoyama, T., additional, Hirata, T., additional, and Terakado, K., additional

Published
2020
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7. Problem of Iron Isotope Composition of the Earth and Moon. Data on δ57Fe of Luna 16, Luna 20, and Luna 24 Lunar Soil Samples (Report on the XXII Symposium on the Geochemistry of Stable Isotopes, Moscow, October 29–31, 2019).

Author

Galimov, E. M., Okabayashi, S., Yokoyama, T., Hirata, T., and Terakado, K.

Subjects
IRON isotopes, LUNAR soil, STABLE isotopes, EARTH'S mantle, EARTH'S core, CHONDRITES, LUNAR craters
Abstract

The model of the formation of the Earth–Moon system during the compression and fragmentation of a gas–dust cloud (Galimov, 2011; Galimov and Krivtsov, 2012) suggests an unusual mechanism for the formation of the Earth's core. In particular, the model predicts that iron in the Earth's core should be enriched in the light isotope, and the Earth's mantle should be, conversely, enriched in the heavy isotope compared to the primary iron (of chondrites). The alternative (megaimpact) model does not allow for this phenomenon. This problem could be solved by comparing the iron isotope composition of the Earth's and Moon's mantles. The best representation of the iron isotope composition of the lunar mantle (δ57Fe) is given by the Fe isotope composition of lunar basalts with very low titanium content (VLT), just as the best representation of the isotope composition of iron in the Earth's mantle is given by the δ57Fe of the Earth's mid-oceanic ridge basalts (MORB). VLT basalts are relatively scarce on the lunar surface, unlike high-titanium basalts, which fill lunar lowlands. Their iron isotope composition has not yet been measured. We were the first to analyze the iron isotope composition of very low-titanium lunar basalts (VLT) in material delivered by the Luna 24 space mission. Our data indicate that the δ57Fe of Earth's mantle is higher than the δ57Fe of the bulk silicate Moon, which means (with a high degree of probability) that the Earth's core is enriched in the light iron isotope. This, in turn, is in good agreement with the model of formation of the Earth–Moon system by the compression and fragmentation of the gas–dust cloud. [ABSTRACT FROM AUTHOR]

Published
2020
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10. Effects of Se1 gene on basic vegetative growth of rice

Author

Niwa, M., Terakado, K., and Takeda, N.

Subjects
Genes, Heading date, Photoperiod, Growth, Chromosomes
Abstract

This article 'Effects of Se1 gene on basic vegetative growth of rice' appeared in the International Rice Research Notes series, created by the International Rice Research Institute (IRRI) to expedite communication among scientists concerned with the development of improved technology for rice and rice-based systems. The series is a mechanism to help scientists keep each other informed of current rice research findings. The concise scientific notes are meant to encourage rice scientists to communicate with one another to obtain details on the research reported.

Published
1996
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15. Marked Depletion of the Water-Channel Protein, AQP5, in the Canine Nictitating Membrane Glands Might Contribute to the Development of KCS.

Author

Terakado, K., Yogo, T., Kohara, Y., Soeta, S., Nezu, Y., Harada, Y., Hara, Y., Amasaki, H., and Tagawa, M.

Subjects
KERATOCONJUNCTIVITIS sicca, DIAGNOSIS of dog diseases, IMMUNOHISTOCHEMISTRY, AQUAPORINS, STAINS & staining (Microscopy)
Abstract

The objectives of this study were to investigate the normal histological localization of aquaporin (AQP) 5 protein in the lacrimal and nictitating membrane glands and to compare this localization in healthy and keratoconjunctivitis sicca (KCS) dogs. Lacrimal and nictitating membrane glands of 5 healthy Beagles and nictitating membrane glands of 5 KCS dogs (3 Beagles and 2 mongrel dogs: 0–13 years) were used for the present study. The owners of the KCS dogs did not consent to perform biopsies of the lacrimal glands. The localization and distribution of AQP5 protein were investigated by an immunohistochemical technique. In immunohistochemical staining, AQP5 was localized in the apical site of acinar epithelial and ductal epithelial cells from both the lacrimal and nictitating membrane glands in healthy dogs. However, AQP5 was not detected in the 5 KCS dogs. These results for immunohistochemical AQP5 localization might correlate with the deficiency in tear secretion found in KCS dogs. [ABSTRACT FROM AUTHOR]

Published
2013
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17. Improving reactivity of naphthalimide-based GST probe by imparting TPP cation: Development and application for live cell imaging.

Author

Fujikawa Y, Terakado K, Nezu S, Noritsugu K, Maemoto Y, Ito A, and Inoue H

Subjects
Mitochondria, Cations, Naphthalimides pharmacology, Glutathione Transferase chemistry
Abstract

Glutathione S-transferases (GSTs) are a superfamily of multifunctional enzymes comprising multiple classes and subtypes. This paper describes the synthesis and characterization of TPPBN-1, a naphthalimide derivative conjugated with a triphenylphosphonium (TPP) cation. When 4-bromonaphthalimide (BrNaph), a previously characterized GST substrate, was conjugated to a TPP cation, the conjugate showed increased reactivity towards most alpha- and mu-class GSTs, particularly the GSTA2 subtype, compared to the parent compound, but hardly towards Pi-class GSTs. Using this probe with enhanced reactivity, the enzymatic activity of endogenous GSTA1/2 in HepG2 cells was visualized by confocal fluorescence microscopy. The results demonstrated that modification with TPP cations, which are often used as tags for targeting mitochondria, can be used to enhance the reactivity of probes for specific GST subtypes., Competing Interests: Declaration of Competing Interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2022. Published by Elsevier Ltd.)

Published
2023
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18. Versatile control of the superconducting transition temperature in anti-ThCr 2 Si 2 -type Y 2 O 2 Bi via H, Li, or F doping.

Author

Terakado K, Kawasoko H, and Fukumura T

Abstract

In Y 2 O 2 Bi with Bi square net, H substitution and Li intercalation led to higher superconducting transition temperature ( T c ), while F substitution led to lower T c , where T c is universally scaled by unit cell tetragonality c / a . Li intercalated Y 2 O 2 Bi showed a higher T c than previously reported Y 2 O 2 Bi even for the similar c / a .

Published
2022
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19. Tetragonality induced superconductivity in anti-ThCr 2 Si 2 -type RE 2 O 2 Bi (RE = rare earth) with Bi square nets.

Author

Sei R, Kawasoko H, Matsumoto K, Arimitsu M, Terakado K, Oka D, Fukuda S, Kimura N, Kasai H, Nishibori E, Ohoyama K, Hoshikawa A, Ishigaki T, Hasegawa T, and Fukumura T

Abstract

We report a series of layered superconductors, anti-ThCr 2 Si 2 -type RE 2 O 2 Bi (RE = rare earth), composed of electrically conductive Bi square nets and magnetic insulating RE 2 O 2 layers. Superconductivity was induced by separating the Bi square nets as a result of excess oxygen incorporation, irrespective of the presence of magnetic ordering in RE 2 O 2 layers. Intriguingly, the transition temperature of all RE 2 O 2 Bi including nonmagnetic Y 2 O 2 Bi was approximately scaled by unit cell tetragonality (c/a), implying a key role in the relative separation of the Bi square nets to induce superconductivity.

Published
2020
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20. 4-Bromo-1,8-naphthalimide derivatives as fluorogenic substrates for live cell imaging of glutathione S-transferase (GST) activity.

Author

Fujikawa Y, Terakado K, Nampo T, Mori M, and Inoue H

Subjects
Cell Line, Tumor, Enzyme Assays methods, Fluorescent Dyes chemical synthesis, Fluorescent Dyes toxicity, Glutathione S-Transferase pi chemistry, Humans, Kinetics, Microscopy, Confocal methods, Microscopy, Fluorescence methods, Naphthalimides chemical synthesis, Naphthalimides toxicity, Neoplasms diagnosis, Fluorescent Dyes chemistry, Glutathione S-Transferase pi analysis, Naphthalimides chemistry
Abstract

Fluorogenic substrates are used to visualize the activity of cancer-associated enzymes and to interpret biological events. Certain types of glutathione S-transferase (GST), such as Pi class GST (referred to as GSTP1), are more highly expressed in a wide variety of human cancer tissues compared to their corresponding normal tissues. Pi class GST is thus a cancer cell molecular marker and potential target for overcoming resistance to chemotherapy. Here, we report that 4-bromo-1,8-naphthalimide (BrNaph) is a practical fluorogenic GST substrate. We have found that HE-BrNaph, an N-hydroxyethyl derivative, shows remarkable fluorescence enhancement upon GST-catalyzed S N Ar replacement of the bromo group with a glutathionyl group. This substitution was highly selective and occurred only in the presence of GSH/GSTs; no non-enzymatic reaction was observed. We demonstrated that HE-BrNaph allows visualization of GST activity in living cells and enables to distinguish cancer cells from normal cells. Further, various N-substitutions in BrNaph retain susceptibility to enzymatic activity and isozyme selectivity, suggesting the applicability of BrNaph derivatives. Thus, BrNaph and its derivatives are GST substrates useful for fluorescence imaging and the intracellular detection of GSTP1 activity in living cells., (Copyright © 2019 Elsevier B.V. All rights reserved.)

Published
2019
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21. Superconductivity in Anti-ThCr 2 Si 2 -type Er 2 O 2 Bi Induced by Incorporation of Excess Oxygen with CaO Oxidant.

Author

Terakado K, Sei R, Kawasoko H, Koretsune T, Oka D, Hasegawa T, and Fukumura T

Abstract

Recently, superconductivity was induced by expanding interlayer distance between Bi square nets in anti-ThCr 2 Si 2 -type Y 2 O 2 Bi through incorporation of excess oxygen with increased nominal amount of oxygen. However, such oxygen incorporation was applicable to only Y 2 O 2 Bi among R 2 O 2 Bi ( R = rare earth metal), probably due to a larger amount of oxygen incorporation for Y 2 O 2 Bi. In this study, the interlayer distance in Er 2 O 2 Bi was increased by cosintering with CaO, which served as an oxidant, indicating that excess oxygen was incorporated in Er 2 O 2 Bi. As a result, superconductivity was induced in Er 2 O 2 Bi at 2.2 K.

Published
2018
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22. Mansonone E from Mansonia gagei Inhibited α-MSH-Induced Melanogenesis in B16 Cells by Inhibiting CREB Expression and Phosphorylation in the PI3K/Akt Pathway.

Author

Nishina A, Miura A, Goto M, Terakado K, Sato D, Kimura H, Hirai Y, Sato H, and Phay N

Subjects
Animals, Cell Line, Tumor, Cell Survival drug effects, Cyclic AMP Response Element-Binding Protein metabolism, Mice, Phosphatidylinositol 3-Kinases metabolism, Phosphorylation drug effects, Plant Bark, Plant Extracts, Proto-Oncogene Proteins c-akt metabolism, Signal Transduction drug effects, Malvaceae, Melanins metabolism, Melanoma, Experimental metabolism, Naphthoquinones pharmacology, Sesquiterpenes pharmacology, alpha-MSH antagonists & inhibitors
Abstract

Many natural products that inhibit melanogenesis, freckles, and hyperpigmentation have been selectively used in cosmetics because melanogenesis is linked to the multiple biogenesis cascades of melanin synthesis. However, some of these compounds have side effects that may result in their restriction in the future. We report here the isolation and structural elucidation of compounds extracted from Mansonia gagei and evaluate their activity on melanogenesis inhibition. We isolated five known compounds from M. gagei and identified them as mansonone E (1), mansorin I (2), populene F (3), mansonone G (4), and mansorin B (5). After evaluating the five compounds for cytotoxicity against B16 cells and inhibitory activity on α-melanocyte-stimulating hormone (α-MSH) induced melanogenesis, we determined that the cytotoxicity and melanogenesis-inhibitory effect of 1 were relatively low and high, respectively. Next, the effect of 1 on the expression of melanogenesis-related proteins was assessed; it was confirmed that 1 dose-dependently inhibited the expression levels of tyrosinase, tyrosinase-related protein 1 (TRP-1), TRP-2, cAMP response element binding protein (CREB), and microphthalmia-associated transcription factor (MITF) which were increased after stimulation by α-MSH. Furthermore, the effects of 1 on the phosphorylation levels of intracellular signaling pathway-related proteins were evaluated, and it was found that 1 dose-dependently rescued the phosphorylation of Akt and p38 mitogen-activated protein kinases (MAPK), which were up- or down-regulated after stimulation by α-MSH. In contrast, treatment with the phosphoinositide 3-kinase (PI3K)/Akt inhibitor wortmannin enhanced melanogenesis inhibition by mansonone E. Cumulatively, the data suggest that 1 suppresses α-MSH-induced melanogenesis in B16 cells by inhibiting both phosphorylation in the PI3K/Akt pathway and the expression of melanogenesis-related proteins.

Published
2018
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23. Fundus photography with a smartphone in indirect ophthalmoscopy in dogs and cats.

Author

Kanemaki N, Inaniwa M, Terakado K, Kawarai S, and Ichikawa Y

Subjects
Animals, Cats, Dogs, Ophthalmoscopy methods, Photography instrumentation, Fundus Oculi, Ophthalmoscopy veterinary, Photography veterinary, Smartphone instrumentation
Abstract

Objective: To introduce a simple method for fundus photography of dogs and cats using a smartphone and indirect ophthalmoscopy lenses., Methods: Fundus photographs of dogs and cats with transparent ocular media were obtained with 15D, 20D, 28D, and 40D indirect lenses and an iPhone-6, in a dark room and after pharmacologic pupil dilation. The photographs were recorded as still images using a video application and a video-to-still image application. Two types of neutral density (ND) filters were used as required for reduction of the torch illumination power of the iPhone., Results: The images obtained in this study were upside-down as a result of the optics used. A 180-degree rotation was used to show their natural anatomical orientation. The image field of view varied with the diopter strength of the indirect lens used. The 40-diopter lens offered the widest field., Conclusion: Still images obtained with a smartphone, and indirect lenses may be useful for client communication and teaching in small animal ophthalmology., (© 2016 American College of Veterinary Ophthalmologists.)

Published
2017
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24. Conjunctival expression of the P2Y2 receptor and the effects of 3% diquafosol ophthalmic solution in dogs.

Author

Terakado K, Yogo T, Kohara Y, Soeta S, Nezu Y, Harada Y, Hara Y, Amasaki H, and Tagawa M

Subjects
Animals, Ophthalmic Solutions, Receptors, Purinergic P2Y2 genetics, Conjunctiva metabolism, Dogs metabolism, Polyphosphates pharmacology, Purinergic P2Y Receptor Agonists pharmacology, Receptors, Purinergic P2Y2 metabolism, Uracil Nucleotides pharmacology
Abstract

Conjunctival epithelial and goblet cell P2Y2 nucleotide receptors regulate ion transport and secretory function. Diquafosol is a P2Y2 purinergic receptor agonist that stimulates secretion of aqueous tear components from conjunctival epithelial cells and secretion of mucin from conjunctival goblet cells. In humans suffering from keratoconjunctivitis sicca (dry eye), topical administration of diquafosol improves corneal epithelial integrity and stabilises the tear film. The aim of the present study was to investigate P2Y2 receptor expression and to determine the effect of topical administration of diquafosol on mucin and aqueous tear production in dogs. Canine conjunctival P2Y2 receptor expression was evaluated by Western blotting and immunohistochemical analysis. The effect of diquafosol on mucin secretion was evaluated by examining mucin-5 subtype AC (MUC5AC) concentration in tears. The effect of diquafosol on aqueous secretions was evaluated by performing the Schirmer tear test (STT) and phenol red thread test. Expression of the P2Y2 receptor was confirmed in canine bulbar and palpebral conjunctivae and receptors were identified at the conjunctival epithelial and goblet cell surface. Tear MUC5AC concentration significantly increased after administration of 3% diquafosol ophthalmic solution, although neither STT nor phenol red thread test values showed any significant change after diquafosol instillation. Topical ocular administration of 3% diquafosol might improve corneal epithelial disorders in dogs through stabilisation of the tear film, by virtue of an increase in MUC5AC secretion., (Copyright © 2014 Elsevier Ltd. All rights reserved.)

Published
2014
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25. Efficacy of the use of a colorimetric pupil light reflex device in the diagnosis of fundus disease or optic pathway disease in dogs.

Author

Terakado K, Yogo T, Nezu Y, Harada Y, Hara Y, and Tagawa M

Subjects
Animals, Blindness diagnosis, Blindness pathology, Dog Diseases diagnosis, Dogs, False Negative Reactions, False Positive Reactions, Female, Male, Predictive Value of Tests, Retinal Degeneration diagnosis, Retinal Degeneration pathology, Retrospective Studies, Sensitivity and Specificity, Blindness veterinary, Dog Diseases pathology, Optic Nerve pathology, Reflex, Pupillary physiology, Retinal Degeneration veterinary
Abstract

The aim of this study was to determine the efficacy of a colorimetric pupil light reflex (PLR) device (Melan-100(®), U.S.A.) in dogs with sudden acquired retinal degeneration syndrome (SARDS; 16 cases), progressive retinal atrophy (PRA; 10 cases) and optic pathway disease (6 cases). The colorimetric device detected PLR abnormality in 32, 16 and 9 eyes with SARDS, PRA and optic pathway disease, respectively, whereas white light detected PLR abnormality in 18, 11 and 9 eyes with SARDS, PRA and optic pathway disease, respectively. SARDS dogs displayed miosis, while optic pathway disease dogs displayed mydriasis in a blue light examination. Thus, colorimetric PLR may be a useful method for determining whether electroretinography (ERG) or magnetic resonance imaging (MRI) should be performed for dogs with acute blindness.

Published
2013
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26. Two novel gonadotropin-releasing hormones (GnRHs) from the urochordate ascidian, Halocynthia roretzi: implications for the origin of vertebrate GnRH isoforms.

Author

Hasunuma I and Terakado K

Subjects
Amino Acid Sequence, Animals, Base Sequence, Evolution, Molecular, Molecular Sequence Data, Phylogeny, Protein Isoforms, Gonadotropin-Releasing Hormone classification, Gonadotropin-Releasing Hormone metabolism, Urochordata metabolism, Vertebrates physiology
Abstract

Three forms of gonadotropin-releasing hormone (GnRH) are found in vertebrates; these differ in amino acid sequence, localization, distribution, and embryological origin. We used northern blot analysis, and in situ hybridization to detect GnRH transcripts in various tissues in the large ascidian Halocynthia roretzi. We cloned a cDNA encoding two novel GnRHs, termed tGnRH-10 and tGnRH-11, from H. roretzi, with deduced amino acid sequences of QHWSYGFSPG and QHWSYGFLPG, respectively. Both GnRHs are highly similar to those of teleosts and tetrapods. For example, the tGnRH-10 sequence is 90% identical to seabream GnRH1, and tGnRH-11 is 90% identical to salmon GnRH3. The primary structure of the deduced preprotein is similar to that of chordate GnRHs and consists of a signal peptide, two decapeptides, up- and downstream processing sequences (containing lysine and arginine), and a GnRH-associated peptide. The transcripts of the H. roretzi GnRH gene were expressed in all tissues examined. Comparison of the signal peptide of the lamprey GnRH-II precursor with those of three forms from representative vertebrates revealed homology to GnRH2 precursors. These novel ascidian GnRHs offer a new perspective on the origin of vertebrate GnRH subtypes. We hypothesize that gnathostome GnRH2 was derived only from lamprey GnRH-II and that ancestral gnathostome GnRH, which produces neurons that originate in peripheral organs, gave rise to vertebrate GnRH1 and GnRH3 through whole-genome duplication.

Published
2013
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27. Impact of site-directed mutant luciferase on quantitative green and orange/red emission intensities in firefly bioluminescence.

Author

Wang Y, Akiyama H, Terakado K, and Nakatsu T

Subjects
Animals, Luciferases, Firefly analysis, Luminescent Measurements, Mutagenesis, Site-Directed, Structure-Activity Relationship, Color, Fireflies enzymology, Fireflies genetics, Luciferases, Firefly chemistry, Luciferases, Firefly genetics
Abstract

Firefly bioluminescence has attracted great interest because of its high quantum yield and intriguing modifiable colours. Modifications to the structure of the enzyme luciferase can change the emission colour of firefly bioluminescence, and the mechanism of the colour change has been intensively studied by biochemists, structural biologists, optical physicists, and quantum-chemistry theorists. Here, we report on the quantitative spectra of firefly bioluminescence catalysed by wild-type and four site-directed mutant luciferases. While the mutation caused different emission spectra, the spectra differed only in the intensity of the green component (λmax ~ 560 nm). In contrast, the orange (λmax ~ 610 nm) and red (λmax ~ 650 nm) components present in all the spectra were almost unaffected by the modifications to the luciferases and changes in pH. Our results reveal that the intensity of the green component is the unique factor that is influenced by the luciferase structure and other reaction conditions.

Published
2013
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28. Case reports of orthodontic treatment of maxillary central incisors with short roots.

Author

Katada H, Terakado K, and Sueishi K

Subjects
Adolescent, Cephalometry, Child, Female, Humans, Incisor diagnostic imaging, Maxilla diagnostic imaging, Radiography, Tooth Extraction adverse effects, Incisor abnormalities, Orthodontics, Corrective methods, Tooth Extraction methods
Abstract

Maxillary central incisors with short roots are occasionally encountered during orthodontic diagnosis. From an esthetic point of view, the central incisors occupy the most noticeable position in the maxillary and mandibular arches, and whether or not to extract them marks a major turning point in the planning of orthodontic treatment. In deciding a treatment strategy in this situation, there are two options to be considered: 1) treatment without extraction due to esthetic considerations; or 2) extraction, taking risk and prognosis into account. Whichever strategy is adopted, however, it will still be necessary to bear in mind that the treatment and prognosis will differ from that in normal orthodontic treatment. If no extraction is to be carried out, care must be taken that no further shortening occurs during the course of active treatment and that stable retention is preserved. On the other hand, if the central incisors are to be extracted, care must be taken to ensure that this has no negative esthetic impact, either during or after orthodontic treatment.

Published
2012
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29. Impaired insulin secretion from the pancreatic islets of hypothyroidal growth-retarded mice.

Author

Taguchi Y, Tasaki Y, Terakado K, Kobayashi K, Machida T, and Kobayashi T

Subjects
Animals, Bodily Secretions drug effects, Glucose pharmacology, Glucose Tolerance Test, Glucose Transporter Type 2 metabolism, Growth Disorders etiology, Hypothyroidism complications, Hypothyroidism drug therapy, Immunohistochemistry, Insulin Secretion, Insulin-Secreting Cells pathology, Mice, Microscopy, Immunoelectron, Polymerase Chain Reaction, Potassium Chloride pharmacology, RNA, Messenger metabolism, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Sulfotransferases genetics, Triiodothyronine administration & dosage, Triiodothyronine pharmacology, Growth Disorders metabolism, Hypothyroidism metabolism, Insulin metabolism, Insulin-Secreting Cells metabolism, Sulfotransferases metabolism
Abstract

The growth-retarded (grt) mouse shows thyroid dysfunction-related hyporesponsiveness to TSH. Thyroid hormone is a critical regulator of metabolism in many cells; thus, derangement of thyroid function affects many organs and systems. Experiments were conducted focusing on the function of the pancreatic islets in grt mice. We showed occurrence of a fasting hyperglycemia and a decreased plasma insulin level response to a glucose load in grt mice, despite normal insulin molecules being stored in secretory granules of pancreatic islets. We also demonstrated a reduction of insulin secretion in response to glucose administration from islets of grt mice in vitro, while the insulin release in response to KCl stimulation was comparable to that in normal mice, indicating that the isolated islets from grt mice have normal ATP-sensitive K(+) channels and postchannel activity. The mRNA expression levels of glucose transporter 2 and glucokinase in the islets of grt mice were similar to those in normal mice. Triiodothyronine administration to grt mice improved insulin secretion very slightly. On the other hand, mRNA for tyrosylprotein sulfotransferase 2 (Tpst2) was found to be expressed in the pancreatic islets of grt mice. Considering that Tpst2 is the responsible gene of grt mice, mutation of which is associated with a poor function of TSH receptor, the findings raise a possibility of involvement of factors including Tpst2 in the insulin hyposecretion in grt mice.

Published
2010
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30. Generation of prolactin-like neurons in the dorsal strand of ascidians.

Author

Terakado K

Subjects
Animals, Gonadotropin-Releasing Hormone metabolism, Urochordata growth & development, Neurons physiology, Prolactin metabolism, Urochordata anatomy & histology, Urochordata physiology
Abstract

The adult ascidian neural complex forms from a thin tube called the neurohypophyseal duct and from the primordium of the cerebral ganglion from the sensory vesicle in metamorphosing larvae. Neurohypophyseal duct cells, located in the anterior left side of the sensory vesicle of swimming larvae, are derived from the anterior embryonic neural plate, which expresses common transcription factors in vertebrates and urochordates. The cerebral ganglion primordium is probably derived from the posterior sensory vesicle during metamorphosis. After metamorphosis begins, the duct elongates anteriorly and fuses with the stomodeal ectoderm, where the dorsal tubercle, a large ciliated structure that opens into the upper part of the pharynx, later develops. The rudiment of the cerebral ganglion and the duct elongate posteriorly. The duct also differentiates into the neural gland. The dorsal wall of the neural gland in adult ascidians has a thick epithelium (placode), the central part of which forms the dorsal strand by repeated invaginations along the visceral nerve. Both gonadotropin-releasing hormone (GnRH) neurons and prolactin-like (non-GnRH) neurons are generated in the dorsal strand and migrate to the cerebral ganglion along the visceral nerve throughout adulthood. Thus, the epithelium derived from the neurohypophyseal duct possesses neurogenic potential to generate neural stem cells of the central (cerebral ganglion) and peripheral (dorsal strand) nervous systems. The generation of prolactin-like neurons and their migration into the brain with GnRH neurons suggest that the ascidian dorsal strand is homologous to the craniate olfactory placode, and provide unequivocal support for the existence of the clade Olfactores.

Published
2010
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31. Deleting two C-terminal alpha-helices is effective to crystallize the bacterial ABC transporter Escherichia coli MsbA complexed with AMP-PNP.

Author

Terakado K, Kodan A, Nakano H, Kimura Y, Ueda K, Nakatsu T, and Kato H

Subjects
ATP-Binding Cassette Transporters metabolism, Adenylyl Imidodiphosphate metabolism, Amino Acid Sequence, Bacterial Proteins metabolism, Crystallography, X-Ray, Escherichia coli metabolism, Models, Molecular, Molecular Sequence Data, Protein Binding, Protein Structure, Quaternary, Protein Structure, Secondary, Protein Structure, Tertiary, Sequence Alignment, ATP-Binding Cassette Transporters chemistry, Adenylyl Imidodiphosphate chemistry, Bacterial Proteins chemistry, Escherichia coli chemistry
Abstract

An MsbA deletion mutant DeltaC21 that lacks the two C-terminal alpha-helices was expressed in Escherichia coli strain C41 and purified by metal-affinity and gel-filtration chromatography. Purified DeltaC21 retained 26% of the activity of the wild-type ATPase and had a similar binding affinity to fluorescent nucleotide derivatives. Although crystals of wild-type MsbA complexed with adenosine 5'-(beta,gamma-imido)triphosphate could not be obtained, crystals of DeltaC21 that diffracted to 4.5 A resolution were obtained. The preliminary DeltaC21 structure had the outward-facing conformation, in contrast to the previously reported E. coli MsbA structure. This result suggests that deletion of the C-terminal alpha-helices may play a role in facilitating the outward-facing nucleotide-bound crystal structure of EcMsbA.

Published
2010
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32. Improved expression and purification of human multidrug resistance protein MDR1 from baculovirus-infected insect cells.

Author

Kodan A, Shibata H, Matsumoto T, Terakado K, Sakiyama K, Matsuo M, Ueda K, and Kato H

Subjects
ATP Binding Cassette Transporter, Subfamily B, Member 1 genetics, Animals, Baculoviridae genetics, Buffers, Cell Line, Cell Membrane chemistry, Enzyme Stability, Humans, Insecta, ATP Binding Cassette Transporter, Subfamily B, Member 1 isolation & purification, ATP Binding Cassette Transporter, Subfamily B, Member 1 metabolism, Baculoviridae metabolism
Abstract

Multidrug resistance protein MDR1 (P-glycoprotein/ABCB1) is an ATP-dependent efflux pump for various cytotoxic agents, and is implicated in the resistance of human tumors to chemotherapeutic drugs. To achieve the three-dimensional structural analysis for its mechanistic implications, large amounts of high-quality and homogeneous MDR1 protein are essential. Here we report a cost-effective method for large-scale expression of human MDR1 using a baculovirus/insect expressSF+ cell system and an alterative purification method to maintain MDR1 in a monodispersed state. After extensively optimizing the detergent, pH, and additives, a high yield (2.8 mg/L) of purified MDR1 was obtained by immobilized metal chelate affinity and size-exclusion chromatographies with 49% recovery. The purified MDR1 exhibited specific ATP hydrolase activity (1.7 micromol/min/mg) in the presence of a substrate, verapamil. This value was 14-fold greater than the basal activity without the drug. Size-exclusion chromatography analysis of purified MDR1 showed a monodispersed elution profile. The present purification method provides suitable material for structural and functional studies on human MDR1.

Published
2009
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33. Placode formation and generation of gonadotropin-releasing hormone (GnRH) neurons in ascidians.

Author

Terakado K

Subjects
Animals, Neurogenesis, Urochordata physiology, Urochordata ultrastructure, Gonadotropin-Releasing Hormone metabolism, Neurons physiology, Urochordata metabolism
Abstract

Neurogenic placodes, a chordate innovation, generate several neuronal populations, including gonadotropin-releasing hormone (GnRH) neurons which are crucial for vertebrate and solitary ascidian urochordate reproduction. The dorsal strand placode of ascidians Is derived from the anterior ridge of the embryonic neural plate and thus shares a common developmental origin and expression of various transcription factors with vertebrate placodes. Despite their importance for understanding vertebrate origins, the evolutionary and developmental origins of the neurogenic placode remain obscure. Here I demonstrate the formation of an elaborate neurogenic placode, which forms the dorsal strand, on part of the neural gland epithelium in a solitary ascidian urochordate, Halocynthia roretzi. Two modes of GnRH neurogenesis in the dorsal strand (a peripheral organ) and the migration of GnRH neurons into the brain along the visceral nerve are also described. Ontogenetically, GnRH neurons are first detected in the dorsal strand and cerebral ganglion of very young Juveniles at almost the same time, demonstrating that ascidians possess morphological and developmental features in common with vertebrates. These results further indicate that the onset of peripheral GnRH neurogenesis and the ability of neurons to migrate into the brain predate the divergence of ascidians and vertebrates. Thus, based on the generation of GnRH neurons, the dorsal strand in ascidians may be homologous to the vertebrate olfactory placode. These organs are derived from the anterior region of the embryonic neural plate, which expresses several transcription factors that invertebrate chordates and vertebrates have in common. These results provide unequivocal support for the clade Olfactories (tunicates + vertebrates).

Published
2009
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34. Molecular characterization and antifungal activity of a family 46 chitosanase from Amycolatopsis sp. CsO-2.

Author

Saito A, Ooya T, Miyatsuchi D, Fuchigami H, Terakado K, Nakayama SY, Watanabe T, Nagata Y, and Ando A

Subjects
Actinomycetales genetics, Chitinases genetics, Chitinases metabolism, Chitosan metabolism, Cloning, Molecular, Escherichia coli enzymology, Escherichia coli genetics, Mutagenesis, Site-Directed, Mutation, Recombinant Proteins genetics, Recombinant Proteins metabolism, Sequence Analysis, DNA, Actinomycetales enzymology, Antifungal Agents pharmacology, Fungal Proteins chemistry, Fungal Proteins genetics, Fungal Proteins metabolism, Glycoside Hydrolases biosynthesis, Glycoside Hydrolases chemistry, Glycoside Hydrolases genetics, Rhizopus drug effects
Abstract

An actinomycete strain, Amycolatopsis sp. CsO-2, produces a 27-kDa chitosanase. To reveal the molecular characteristics of the enzyme, its corresponding gene ctoA was cloned by a reverse genetic technique, based on the N-terminal amino acid sequence of the protein. The encoded CtoA protein was deduced to be composed of 286 amino acids, including a putative signal peptide (1-48), and exhibited 83% identity in the amino acid sequence with the family 46 chitosanases from Streptomyces sp. N174 or Nocardioides sp. N106. The active recombinant CtoA protein was successfully overproduced in Escherichia coli. The mutant protein E22Q, in which the glutamic acid residue 22 was replaced with glutamine, abolished the chitosanase activity, showing that the Glu22 residue is required for the enzymatic activity. CtoA exhibited antifungal activity against Rhizopus oryzae, which is known to produce chitosan probably as a cell wall component. In contrast, E22Q did not inhibit the growth of the fungus, suggesting that chitosan-hydrolyzing activity is essential for the antifungal activity. It is noteworthy that the antifungal effect of CtoA against R. oryzae was drastically enhanced by the simultaneous addition of the family 19 chitinase ChiC from Streptomyces griseus.

Published
2009
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35. Dynamic mechanism for the serpin loop insertion as revealed by quantitative kinetics.

Author

Takahashi N, Terakado K, Nakamura G, Soekmadji C, Masuoka T, Yamasaki M, and Hirose M

Subjects
Animals, Chickens, Hydrogen-Ion Concentration, Kinetics, Mutation genetics, Ovalbumin chemistry, Ovalbumin genetics, Protein Binding, Protein Denaturation, Subtilisin metabolism, Temperature, Thermodynamics, Ovalbumin metabolism, Serpins metabolism
Abstract

The serpin conformational change by insertion of the reactive center loop into beta-sheet A plays a central role in multiple physiological consequences such as serine proteinase inhibition, latency and serpinopathic polymerization. To study the dynamic mechanism for the loop insertion, a novel kinetic method was established utilizing the ovalbumin mutant R339T/A352R; the loop insertion progressed after the cleavage of P1-P1' (Arg352-Ser353) by trypsin was quenched at pH 8 and 0.5 degrees C, and different conformers were quantified by separation using ion-exchange HPLC. The apparent first-order rate constant k(app) determined for various R339T/A352R derivatives differing in conformational stability was greatly increased by lowering the pH. The pH-dependence of k(app) indicated that the protonation of side-chain(s) with a pK(a) value of around 4.6 is a pre-requisite for the loop insertion. The theoretical rate constant k for the protonated form calculated from k(app) was highly variable, depending on the ovalbumin derivative; structural modifications that give increased mobility to helix F and the sheet-A half (s3A/s2A/s1A) resulted in a striking increase in the loop insertion rate constant k. The k values were determined at different temperatures for all the ovalbumin derivatives, and DeltaH(double dagger) and DeltaS(double dagger) values for the loop insertion reaction were determined according to the transition theory. The formation of the transition state was highly endothermic with minor entropy gain, requiring a DeltaG(double dagger) larger than 18 kcal/mol, which can offset the hydrogen-bond cleavages between s3A and s5A. These results are consistent with the transition state with an opened sheet A and altered orientation of helix F.

Published
2005
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36. Adrenocorticotropin-like immunoreactivity in the granules of neural complex cells of the ascidian Halocynthia roretzi.

Author

Kawahara G, Terakado K, Sekiguchi T, Inoue K, and Kikuyama S

Subjects
Adrenocorticotropic Hormone immunology, Animals, Immunohistochemistry, Microscopy, Immunoelectron, Nervous System ultrastructure, Secretory Vesicles ultrastructure, Urochordata ultrastructure, Adrenocorticotropic Hormone analysis, Nervous System chemistry, Nervous System cytology, Secretory Vesicles chemistry, Urochordata chemistry, Urochordata cytology
Abstract

Immunohistochemical studies on the neural complex (neural gland, dorsal strand, and cerebral ganglion) of an ascidian, Halocynthia roretzi, were performed by using an antiserum against porcine ACTH. The antiserum recognized a considerable number of the cells scattered along the tubular structure of the dorsal strand and a few cells in the cerebral ganglion. Immunoelectron microscopic studies revealed that the ACTH-like substance resided within secretory granules with diameter of 300-500 nm. Furthermore, those ACTH-immunoreactive cells were demonstrated to be different from PRL-immunoreactive cells, the presence of which had previously been reported.

Published
2002
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37. Induction of gamete release by gonadotropin-releasing hormone in a protochordate, Ciona intestinalis.

Author

Terakado K

Subjects
Animals, Ciona intestinalis drug effects, Ganglia, Invertebrate cytology, Germ Cells drug effects, Gonadotropin-Releasing Hormone administration & dosage, Gonadotropin-Releasing Hormone analysis, Microscopy, Electron, Neurons chemistry, Neurons ultrastructure, Ciona intestinalis physiology, Germ Cells physiology, Gonadotropin-Releasing Hormone pharmacology
Abstract

Gonadotropin-releasing hormone (GnRH) of vertebrates is now believed to have multiple functions in addition to its role as a hypophysiotropic hormone, as originally defined. Recently, it has been shown that GnRH occurs also in the ascidians, which are considered ancestral chordates. Here the author shows that GnRH induces spawning of gametes from mature individuals of Ciona intestinalis. Ciona accumulates mature gametes in the gonoducts and maintains them until spawning is triggered by a photoperiodic cue(s). Injection of synthetic tunicate GnRH-I or -II into various sites of mature individuals effectively induced gamete release (spawning), although the former was more potent. Gamete release often occurred on a larger scale than in spontaneous spawning. However, moderate gamete release, similar to spontaneous spawning, was often triggered by exogenous tunicate GnRH. GnRH in vivo apparently is released from the GnRH-containing neurons that are distributed from the region of the cerebral ganglion to the proximal part of the ovary along the dorsal strand within the blood sinus; this indicates that both forms of tunicate GnRH may be the actual inducers of spawning. It is suggested that, in the ancestral chordate, GnRH neurons release GnRH prior to the spawning and the released GnRH acts directly on the epithelium of gonoducts or functions as a neuromodulator of other neurons innervating the gonoducts to induce spawning.

Published
2001
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38. Test cell migration and tunic formation during post-hatching development of the larva of the ascidian, Ciona intestinalis.

Author

Sato Y, Terakado K, and Morisawa M

Subjects
Animals, Cell Movement, Ciona intestinalis cytology, Ciona intestinalis physiology, Epidermal Cells, Epidermis growth & development, Female, Larva cytology, Larva growth & development, Larva physiology, Male, Metamorphosis, Biological, Microscopy, Electron, Microscopy, Video, Swimming, Ciona intestinalis growth & development
Abstract

Morphological changes in the tunic layers and migration of the test cells during swimming period in the larva of the ascidian, Ciona intestinalis, were observed by light and electron microscopy. The swimming period was divided into three stages. In stage 1, further formation of juvenile tunic layer started only in the larval trunk and neck region. In stage 2, the layer became swollen in the ventral and dorsal sides of the neck region and in stage 3, the swelling expanded backward. Concomitantly with these changes, the outermost larval tunic layer (outer cuticular layer), which had been formed before hatching, also swelled in the neck region in stage 2 and formed two humps in stage 3, although the layer did not change in the tail region during the swimming period. Test cells that were present over the entire larval tunic layer in stage 1 began to move from the surface of the fin toward that of the side of the body in stage 2, and finally gathered to form six bands running radially from the anterior end to the posterior end of the trunk region and aligned along the lateral sides of body in the tail region in stage 3. In electron microscopic observations, pseudopodia protruding from the test cells invaded the larval tunic, following which they extended proximate to the juvenile tunic in the trunk region. In the tail region, which had no juvenile tunic layer as that described, the pseudopodia invaded and remained adjacent to the surface of the epidermis or the sensory cilia protruded from the epidermis. Metamorphosis of the larvae, further tunic formation, degradation of adhesive papilla, attachment of larva to the substratum and tail resorption commenced after these morphological changes occurred. The possible role of the test cells in metamorphosis is discussed.

Published
1997
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39. Formation of amyloid-like fibrils in COS cells overexpressing part of the Alzheimer amyloid protein precursor.

Author

Maruyama K, Terakado K, Usami M, and Yoshikawa K

Subjects
Amyloid beta-Protein Precursor, Animals, Base Sequence, Cell Line, Chlorocebus aethiops, Cloning, Molecular, DNA genetics, Immunoenzyme Techniques, Immunohistochemistry, Inclusion Bodies metabolism, Macromolecular Substances, Microscopy, Electron, Microscopy, Immunoelectron, Molecular Sequence Data, Peptide Fragments genetics, Transfection, Alzheimer Disease metabolism, Amyloid beta-Peptides genetics, Amyloid beta-Peptides metabolism, Gene Expression, Protein Precursors genetics
Abstract

A pathological hallmark of Alzheimer's disease is the deposition of amyloid fibrils in the brain. The principal component of the amyloid fibril is beta/A4 protein, which is derived from a large membrane-bound glycoprotein, Alzheimer amyloid protein precursor (APP). Although the deposition of amyloid is thought to result from the aberrant processing of APP, the detailed molecular mechanisms of amyloidogenesis remain unclear. A C-terminal fragment of APP which spans the beta/A4 and cytoplasmic domains has a tendency to self-aggregate. In an attempt to establish a cultured-cell model for amyloid fibril formation, we have transfected COS-1 cells with complementary DNA encoding the C-terminal 100 residues of APP. In the perinuclear regions of a small population of DNA-transfected cells, we observed inclusion-like deposits which showed a strong immunohistochemical reaction towards an anti-C-terminal APP antibody or an anti-beta/A4 amyloid core-specific antibody. Electron microscope observations of the inclusion-carrying cells revealed an accumulation of amyloid-like fibrils of 8-22 nm diameter near and on the nuclear membrane. The fibrils showed a beaded or helical structure, and reacted positively with the anti-C-terminus antibody by immunoelectron microscopy. These results suggest that the formation of amyloid fibrils is an inherent characteristic of the C-terminal peptide of APP. The present system provides a suitable model for the molecular dissection of the process of brain amyloidogenesis.

Published
1990
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40. Chromatin Arrangement and Axis Formation in the Spermiogenesis of a Pulmonate Snail.

Author

Terakado K

Abstract

Nuclear change in relation to axis formation and condensation during spermiogenesis was investigated in the snail, Physa acuta. In the early spermatid, characteristic thick layers (termed apical and basal plates) are formed on two sides of a nuclear envelope. Soon after the formation of these plates, a developing acrosome and a flagellum attach externally to the center of the apical and basal plates, respectively. However, most (presumably all) of the chromatin filaments become attached all over the inner surface of the apical and basal plates. This means that the plates themselves are actually the specialized forms of the nuclear envelope to which chromatin filaments become connected; by means of these plates, the chromatin filaments become arranged in parallel to the antero-posterior axis as the nucleus elongates. This suggests that the formation of these two thick layers on opposing surfaces of the nucleus primarily determines the antero-posterior axis of the spermatid and the direction of the arrangement of chromatin. The flattening of the nucleus prior to elongation is caused mainly by the enlargement of the basal plate. Subsequent nuclear shaping and condensation are discussed in relation to the change in the surface structures of the nucleus and the organization of the microtubules.

Published
1981
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42. Ultrastructural studies on the formation of yolk granules in the statoblast of a fresh-water bryozoan, Pectinatella gelatinosa.

Author

Terakado K and Mukai H

Abstract

The formation of protein-carbohydrate yolk in the statoblast of a fresh-water bryozoan, Pectinatella gelatinosa, was studied by electron microscopy. Two types (I and II) of yolk cells were distinguished. The type I yolk cells are mononucleate and comprise a large majority of the yolk cells. The type II yolk cells are small in number; they become multinucleate by fusion of cells at an early stage of vitellogenesis. In both types of yolk cells, electron-dense granules (dense bodies) are formed in Golgi or condensing vacuoles, which are then called yolk granules. For the formation of yolk granules, the following processes are considered: 1. Yolk protein is synthesized in the rough-surfaced endoplasmic reticulum (RER) of the yolk cells. 2. The synthesized protein condenses in the cisternal space of the RER and is packaged into small oval swellings, which are then released from the RER as small vesicles (Golgi vesicles, 300-600 A in diameter). 3. The small vesicles fuse with one another to form condensing vacuoles, or with pre-existing growing yolk granules. 4. In the matrix of the condensing vacuoles or growing yolk granules, electron-dense fibers are fabricated and then arranged in a paracrystalline pattern to form the dense body. 5. After the dense body reaches its full size, excess membrane is removed and eventually the yolk granules come to mature. Toward the end of vitellogenesis of the yolk cells, the cytoplasmic organelles are ingested by autophagosomes derived from multivesicular bodies and disappear., (Copyright © 1978 Wiley-Liss, Inc.)

Published
1978
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43. Ultrastructure of the thread cells in the slime gland of Japanese hagfishes, Paramyxine atami and Eptatretus burgeri.

Author

Terakado K, Ogawa M, Hashimoto Y, and Matsuzaki H

Subjects
Animals, Cell Nucleolus ultrastructure, Golgi Apparatus ultrastructure, Histocytochemistry, Mucous Membrane ultrastructure, Organoids ultrastructure, Polyribosomes ultrastructure, Protein Biosynthesis, Ribosomes ultrastructure, Skin ultrastructure, Exocrine Glands ultrastructure, Fishes anatomy & histology, Hagfishes anatomy & histology
Abstract

The thread cells in the slime gland of Japanese hagfishes, Paramyxine atami and Eptatretus burgeri were studied by light and electron microscopy. The mature thread cells are large elements (180 times 80 mu) filled with an intricately coiled thread, approximately 2 mu in diameter. The protein nature of the thread has been confirmed by histochemical examination. In the initial stage of growth, the thread consists of a bundle of distinctly parallel filaments approximately 90-120 A in diameter and a centrally located tubular component approximately 230-260 A in diameter which occurs singly or occasionally as a double and triple structure. The developing thread displays thin filaments, approximately 30-60 A in diameter. The thin filaments are composed of fine fibrous structures, subfilaments, approximately 10-30 A in diameter. On the outer surface of the thread a coating is apparent, giving it a fluffy appearance. Polysomal clusters consisting of five or six ribosomes are predominant. Fine fibrous structures are also found among the threads; they seem to have a spatial relationship with the polysomes and resemble the subfilament constituents of the thin filaments. From these results, it may be suggested that the fine fibrous structures synthesized by polysomes, twist together and coalesce into a thread. The problem of the polysome size and the molecular weight of the fibrous protein synthesized is discussed.

Published
1975
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44. FINE STRUCTURE AND SIZE DISTRIBUTION OF FREE THICK FILAMENTS IN EARLY FIBRILLOGENESIS OF ASCIDIAN TADPOLE.

Author

Terakado K

Abstract

The development and the size distribution of free thick filaments which accumulate in the early stages of myofibril formation in somitic myoblasts of the ascidian tadpole were studied by electron microscopy. Such filaments appeared in the cell cortex but, rather dominantly, the aggregates of these thick filaments and filamentous structures were observed in the interior of the cell. The aggregate consisted of some of the following elements: filamentous structures (20-60 A in diameter); free thick filaments (60-220 A); dense Z-band precursor materials; bundles of thick (140-160 A) and thin (60-70 A) filaments; and ribosomal clusters. The free thick filaments were variable in diameter and showed long lateral projections (300-600 A) and tapered ends. The variation curve in diameter of the free thick filaments indicates a continuous size distribution, suggesting the continuous growth of these filaments by polymerization of myosin molecules. Free thick filaments thicker than myosin filaments which were found within myofibrils were present; their significance is discussed in relation to myosin filament formation.

Published
1975
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45. CYTOLOGICAL AND ULTRASTRUCTURAL STUDIES ON MUSCLE DIFFERENTIATION IN THE ASCIDIAN, PEROPHORA ORIENTALIS*,*.

Author

Terakado K

Abstract

Muscle cell differentiation in the tail of the ascidian, Perophora orientalis, from early tail-bud embryos to swimming larvae, were studied cytologically and ultrastructurally. Myogenic cells did not form multinucleated myotubes, but remained as mononucleated cells. Nucleolar component increased prior to a marked increase in cytoplasmic RNA. Cytoplasmic RNA appeared first around nucleus and later concentrated in the peripheral cytoplasm. The fine filaments measuring 20-30 Å in their thin parts and 30-45 Å in their thick parts in diameter appeared initially, forming loose networks, in the peripheral cytoplasm where ribosome clusters had been concentrated. These filaments were tightly attached by particles of various size and density. These filaments tended to be arranged in parallel as they increased in their size. They seemed to be precursors of both actin and myosin filaments of formed myofibrils. Z band precursors were found as dense patches in association with loosely arranged myofilaments and consisted of particulate and filamentous materials. The myofibrils seemed to grow further by organizing free filaments into bundles and further by aligning bundles of myofilaments at both ends.

Published
1972
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46. THE EFFECTS OF ACTINOMYCIN D ON MUSCLE CELLS OF ASCIDIAN EMBRYO.

Author

Terakado K

Abstract

The effect of actinomycin D on muscle cells development of the ascidian, Herdmania momus was studied ultrastructurally. No myofilament was formed when the drug was given at any stage before early tail-bud stage (stage 3). Some aggregates of myofilaments in various size were formed when the treatment was started at stage 4 (4.5 hr after fertilization at about 28°C). Above 60% of myofibrils of fully differentiated muscle cells were formed when the treatment was initiated at stage 5 (5 hr after fertilization). Muscle cells of the tadpoles treated from stage 7 (6 hr after fertilization), at which myofilaments were first detectable in normal development, differentiated almost normally. It is therefore suggested that most mRNAs for muscle proteins are synthesized preceding the onset of myofilament formation and are relatively stable. It is also suggested that mRNAs for myosin, actin and Z band materials are almost simultaneously synthesized. One of the characteristic features of the muscle cell development of the ascidian embryo is almost synchronous differentiation of relatively small numbers of cells (about 54-60 cells). The significance of these results is discussed in relation to mosaic natures of the muscle development.

Published
1973
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