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Dive into the research topics where A. S. Apu is active.

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Featured researches published by A. S. Apu.


General and Comparative Endocrinology | 2016

Molecular cloning of motilin and mechanism of motilin-induced gastrointestinal motility in Japanese quail.

A. S. Apu; Anupom Mondal; Takio Kitazawa; Shota Takemi; Takafumi Sakai; Ichiro Sakata

Motilin, a peptide hormone produced in the upper intestinal mucosa, plays an important role in the regulation of gastrointestinal (GI) motility. In the present study, we first determined the cDNA and amino acid sequences of motilin in the Japanese quail and studied the distribution of motilin-producing cells in the gastrointestinal tract. We also examined the motilin-induced contractile properties of quail GI tracts using an in vitro organ bath, and then elucidated the mechanisms of motilin-induced contraction in the proventriculus and duodenum of the quail. Mature quail motilin was composed of 22 amino acid residues, which showed high homology with chicken (95.4%), human (72.7%), and dog (72.7%) motilin. Immunohistochemical analysis showed that motilin-immunopositive cells were present in the mucosal layer of the duodenum (23.4±4.6cells/mm(2)), jejunum (15.2±0.8cells/mm(2)), and ileum (2.5±0.7cells/mm(2)), but were not observed in the crop, proventriculus, and colon. In the organ bath study, chicken motilin induced dose-dependent contraction in the proventriculus and small intestine. On the other hand, chicken ghrelin had no effect on contraction in the GI tract. Motilin-induced contraction in the duodenum was not inhibited by atropine, hexamethonium, ritanserin, ondansetron, or tetrodotoxin. However, motilin-induced contractions in the proventriculus were significantly inhibited by atropine and tetrodotoxin. These results suggest that motilin is the major stimulant of GI contraction in quail, as it is in mammals and the site of action of motilin is different between small intestine and proventriculus.


Zoological Science | 2016

Molecular Cloning of Ghrelin and Characteristics of Ghrelin-Producing Cells in the Gastrointestinal Tract of the Common Marmoset (Callithrix jacchus)

Shota Takemi; Ichiro Sakata; A. S. Apu; Shinji Tsukahara; Satowa Yahashi; Goro Katsuura; Fumihiro Iwashige; Atsushi Akune; Akio Inui; Takafumi Sakai

Ghrelin was first isolated from human and rat as an endogenous ligand for the growth hormone secretagogue receptor (GHS-R). In the present study, we determined the ghrelin cDNA sequence of the common marmoset (Callithrix jacchus), a small-bodied New World monkey, and investigated the distribution of ghrelin-producing cells in the gastrointestinal tract and localization profiles with somatostatin-producing cells. The marmoset ghrelin cDNA coding region was 354 base pairs, and showed high homology to that in human, rhesus monkey, and mouse. Marmoset ghrelin consists of 28 amino acids, and the N-terminal region is highly conserved as found in other mammalian species. Marmoset preproghrelin and mature ghrelin have 86.3% and 92.9% homology, respectively, to their human counterparts. Quantitative RT-PCR analysis showed that marmoset ghrelin mRNA is highly expressed in the stomach, but it is not detected in other tissues of the gastrointestinal tract. In addition, a large number of ghrelin mRNA-expressing cells and ghrelin-immunopositive cells were detected in the mucosal layer of the stomach, but not in the myenteric plexus. Moreover, all the ghrelin cells examined in the stomach were observed to be closed-type. Double staining showed that somatostatin-immunopositive cells were not co-localized with ghrelin-producing cells; however, a subset of somatostatin-immunopositive cells is directly adjacent to ghrelin-immunopositive cells. These findings suggest that the distribution of ghrelin cells in marmoset differs from that in rodents, and thus the marmoset may be a more useful model for the translational study of ghrelin in primates. In conclusion, we have clarified the expression and cell distribution of ghrelin in marmoset, which may represent a useful model in translational study.


Iranian Journal of Applied Animal Science | 2012

A Comparative Study of Fresh and Frozen-Thawed Semen Quality in Relation to Fertility of Black Bengal Goats

A. S. Apu; M. A. M. Yahia Khandoker; S. S. Husain; M. Fakruzzaman; D.R. Notter


Bangladesh Journal of Animal Science | 2013

Study on buck evaluation based on semen quality and fertility

F Sultana; S. S. Husain; A. Khatun; A. S. Apu; M. A. M. Y. Khandoker


The Journal of Agricultural Science | 2013

Selection of Black Bengal Buck Based on Some Reproductive Performance of Their Progeny at Semi-Intensive Rearing System

M.N. Haque; S. S. Husain; M. A. M. Y. Khandoker; M.M. Mia; A. S. Apu


Bangladesh Journal of Animal Science | 2012

Investigation On Seminal Attributes And Fertility Of Black Bengal Goat

A. S. Apu; S. S. Husain; M. A. M. Y. Khandoker; A. H. M. S. Rahman; Notter


Bangladesh Journal of Animal Science | 2012

In vitro maturation of buffalo oocytes and fertilization by cattle spermatozoa

M. A. M. Y. Khandoker; M. M. T. Reza; L. Y. Asad; S. Saha; A. S. Apu; S. A. M. Hoque


Journal of The Bangladesh Agricultural University | 2011

A baseline survey on the availability of Black Bengal breeding bucks in different districts of Bangladesh

M. A. M. Y. Khandoker; A. S. Apu; S. S. Husain; D.R. Notter


Archive | 2012

Fertility of Fresh and Frozen-thawed Black Bengal Goat Spermatozoa

A. S. Apu


Bangladesh Journal of Animal Science | 2012

MORPHOMETRIC CHARACTERIZATION AND RELATIONSHIP OF BODY WEIGHT WITH LINEAR BODY MEASUREMENTS IN BLACK BENGAL BUCK

A. H. M. S. Rahman; M. A. M. Y. Khandoker; S. S. Husain; A. S. Apu; A. Mondal; Notter

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M. A. M. Y. Khandoker

Bangladesh Agricultural University

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S. S. Husain

Bangladesh Agricultural University

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A. H. M. S. Rahman

Bangladesh Agricultural University

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A. Mondal

Bangladesh Agricultural University

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M.M. Mia

Bangladesh Livestock Research Institute

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