推荐产品
品質等級
化驗
≥95% (GC)
形狀
powder
mp
41-42 °C (lit.)
溶解度
pyridine: 50 mg/mL, clear, colorless to faintly yellow
螢光
λex 312 nm in methanol
λex 360 nm; λem 449 nm (Reaction product)
儲存溫度
−20°C
SMILES 字串
CCCCCCC(=O)Oc1ccc2C(C)=CC(=O)Oc2c1
InChI
1S/C17H20O4/c1-3-4-5-6-7-16(18)20-13-8-9-14-12(2)10-17(19)21-15(14)11-13/h8-11H,3-7H2,1-2H3
InChI 密鑰
FFNBFZWIBOIPIV-UHFFFAOYSA-N
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儲存類別代碼
11 - Combustible Solids
水污染物質分類(WGK)
WGK 3
閃點(°F)
Not applicable
閃點(°C)
Not applicable
個人防護裝備
Eyeshields, Gloves, type N95 (US)
S Krüger-Krasagakes et al.
Journal of immunological methods, 156(1), 1-8 (1992-11-25)
In order to measure cell mediated cytotoxicity to adherent growing cell lines in vitro more rapidly and conveniently, a fluorometric microassay was developed and results were compared with those obtained by the 51Cr release assay. The fluorometric method is based
L Fiksdal et al.
Applied and environmental microbiology, 55(9), 2424-2427 (1989-09-01)
The production of an enzyme, 4-methylumbelliferyl heptanoate hydrolase, in Escherichia coli exposed to enriched and nonenriched seawater was studied. In all media, except for seawater with no or very small amounts of organic material and seawater enriched with peptone, 4-methylumbelliferyl
E N Dotsika et al.
Journal of immunological methods, 105(1), 55-62 (1987-12-04)
A microplate method for assessing cell growth and viability based on the hydrolysis of fluorogenic substrates by cell esterases has been investigated. Living cells incubated with fluorescein diacetate or 4-methylumbelliferyl heptanoate generate a fluorescent product which is proportional to the
L Virág et al.
Journal of immunological methods, 185(2), 199-208 (1995-09-25)
A fluorimetric method using 4-methylumbelliferyl heptanoate (MUH) has been developed for detecting cell-mediated cytotoxicity and cell proliferation. The assay is based on the hydrolysis of the fluorochrome (MUH) by intracellular esterases of viable cells resulting in the production of highly
R Stadler et al.
The Journal of investigative dermatology, 93(4), 532-534 (1989-10-01)
In the present study we describe a simple technique for the determination of keratinocyte proliferation in vitro, based on the hydrolysis of a fluorogenic substrate by cell esterases. Normal and transformed human keratinocytes were grown in microtiter plates and were
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