Makoto Amano scite author profile

Ethyl acetate extracts from the flowers and leaves of Peroeskiu abrotunoides Karel., Nepetu juncea Benth. and Thymus linearis Benth. growing wild at 2000-3500 in a.s.1. in the Karakoram-Himalaya district were analyzed by GC/MS. The majorvolatileconstituentswere 1,tl-cineole (24.4-27.1%) anda-pinene (18.2-23.2%) for P. abrotunoides, and nepetalactone (71.8%) for N . juncea. Two cheinotypes of T. linearis were found in different area, a thymoll carvacrol type in the areas of Hunza and Rupal Valley, and a geraniollgeranyl acetate type in the area of Rakaposhi Valley. Herbs and their major constituents of N . juncea and T. linearis showed potent antifungal activity by vapor contact, but those of P. abrotanoides showed no significant activity.

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Biosystematic study ofSedum L. SubgenusAizoon (Crassulaceae)

Amano

1990

Bot. Mag. Tokyo

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Development of a practical sandwich assay to detect human pluripotent stem cells using cell culture media

Tateno

Hiemori

Hirayasu³

et al. 2017

Regenerative Therapy

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Human pluripotent stem cells are considered to be ideal cell sources for regenerative medicine, but their clinical and industrial application is hindered by their tumorigenic potential. Previously we have identified a pluripotent stem cell-specific lectin rBC2LCN recognizing podocalyxin as a cell surface ligand. More recently, podocalyxin was found to be a soluble ligand of rBC2LCN that is secreted specifically from human pluripotent stem cells into cell culture media. Taking advantage of this phenomenon, we have previously developed a sandwich assay targeting the soluble podocalyxin using rBC2LCN as a capturing probe and another lectin rABA as an overlay probe to detect human pluripotent stem cells residing in cell therapy products derived from human pluripotent stem cells. A drawback to this, however, was that cell culture media containing fetal bovine serum was found to cause a substantial background signal to the sandwich assay. To reduce the background and increase the sensitivity, we screened different overlay probes to detect the soluble podocalyxin. Among them, an anti-keratan sulfate monoclonal antibody called R-10G showed the highest sensitivity and provided a low background signal to fetal bovine serum. The established sandwich assay using rBC2LCN and R-10G was proved to be powerful, which allowed the high-sensitive detection of human induced pluripotent stem cells residing among clinical-grade cardiomyocytes and neural stem cells, both derived from human induced pluripotent stem cells. The developed method has a possibility to be a standard technology to detect human induced pluripotent stem cells resided in various types of cell therapy products.

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Comparison of the structural characteristics of chromosome VI inSaccharomyces sensu stricto: The divergence, species-dependent features and uniqueness of saké yeasts

Nakazato¹,

Kadokura²,

Amano³

et al. 1998

Yeast

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Previous studies have revealed that chromosome VI of saké yeasts is much larger than that of the other strains of Saccharomyces cerevisiae. Southern analysis using segments of chromosome VI of a laboratory strain as probes suggested that the nucleotide sequence of a major portion of this chromosome is conserved, but considerable diversity was found in the distal parts in the other strains. Physical maps also indicated that differences in length of chromosome VI were mainly due to differences in its ends. NotI was found to generate 9 kb and/or 16 kb fragments from the left telomere of chromosome VI in most saké yeasts, but no fragment in the case of AB972. SfiI produced one or two 30–50 kb fragments from the right end of this chromosome in all saké yeasts tested, but produced a 20 kb fragment in the case of AB972. All S. cerevisiae strains not employed in saké brewing were the same as AB972 in these respects. S. paradoxus had one NotI site in chromosome VI, while S. bayanus had two, one of which is possibly common to both species. The SfiI site mentioned above was present in chromosome VI of all species, while that of S. bayanus and S. paradoxus each had a second site distinct from the other. Chromosome VI of S. pastorianus was not distinguishable from that of S. bayanus. © 1998 John Wiley & Sons, Ltd.

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Makoto Amano

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Volatile Aroma Constituents of Three Labiatae Herbs Growing Wild in the Karakoram-Himalaya District and Their Antifungal Activity by Vapor Contact

Biosystematic study ofSedum L. SubgenusAizoon (Crassulaceae)

Development of a practical sandwich assay to detect human pluripotent stem cells using cell culture media

Comparison of the structural characteristics of chromosome VI inSaccharomyces sensu stricto: The divergence, species-dependent features and uniqueness of saké yeasts

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