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  • 1082737-41-4 Structure
  • Basic information

    1. Product Name: C17H21F5O7
    2. Synonyms: C17H21F5O7
    3. CAS NO:1082737-41-4
    4. Molecular Formula:
    5. Molecular Weight: 432.342
    6. EINECS: N/A
    7. Product Categories: N/A
    8. Mol File: 1082737-41-4.mol
  • Chemical Properties

    1. Melting Point: N/A
    2. Boiling Point: N/A
    3. Flash Point: N/A
    4. Appearance: N/A
    5. Density: N/A
    6. Refractive Index: N/A
    7. Storage Temp.: N/A
    8. Solubility: N/A
    9. CAS DataBase Reference: C17H21F5O7(CAS DataBase Reference)
    10. NIST Chemistry Reference: C17H21F5O7(1082737-41-4)
    11. EPA Substance Registry System: C17H21F5O7(1082737-41-4)
  • Safety Data

    1. Hazard Codes: N/A
    2. Statements: N/A
    3. Safety Statements: N/A
    4. WGK Germany:
    5. RTECS:
    6. HazardClass: N/A
    7. PackingGroup: N/A
    8. Hazardous Substances Data: 1082737-41-4(Hazardous Substances Data)

1082737-41-4 Usage

Check Digit Verification of cas no

The CAS Registry Mumber 1082737-41-4 includes 10 digits separated into 3 groups by hyphens. The first part of the number,starting from the left, has 7 digits, 1,0,8,2,7,3 and 7 respectively; the second part has 2 digits, 4 and 1 respectively.
Calculate Digit Verification of CAS Registry Number 1082737-41:
(9*1)+(8*0)+(7*8)+(6*2)+(5*7)+(4*3)+(3*7)+(2*4)+(1*1)=154
154 % 10 = 4
So 1082737-41-4 is a valid CAS Registry Number.

1082737-41-4Downstream Products

1082737-41-4Relevant articles and documents

Structural requirements for a lipoamino acid in modulating the anticonvulsant activities of systemically active galanin analogues

Zhang, Liuyin,Robertson, Charles R.,Green, Brad R.,Pruess, Timothy H.,White, H. Steve,Bulaj, Grzegorz

, p. 1310 - 1316 (2009)

Introduction of lipoamino acid (LAA), Lys-palmitoyl, and cationization into a series of galanin analogues yielded systemically active anticonvulsant compounds. To study the relationship between the LAA structure and anticonvulsant activity, orthogonally p

Poly(ethylene glycol)-based stable isotope labeling reagents for the quantitative analysis of low molecular weight metabolites by LC-MS

Abello, Nicolas,Geurink, Paul P.,Van Der Toorn, Marco,Van Oosterhout, Antoon J. M.,Lugtenburg, Johan,Van Der Marel, Gijs A.,Kerstjens, Huib A. M.,Postma, Dirkje S.,Overkleeft, Hermen S.,Bischoff, Rainer

experimental part, p. 9171 - 9180 (2009/06/20)

Stable isotope labeling (SIL) in combination with liquid chromatography-mass spectrometry is one of the most widely used quantitative analytical methods due to its sensitivity and ability to deal with extremely complex biological samples. However, SIL methods for metabolite analysis are still often limited in terms of multiplexing, the chromatographic properties of the derivatized analytes, or their ionization efficiency. Here we describe a new family of reagents for the SIL of primary amine-containing compounds based on pentafluorophenyl-activated esters of 13C-containing poly(ethylene glycol) chains (PEG) that addresses these shortcomings. A sequential buildup of the PEG chain allowed the introduction of various numbers of 13C atoms opening extended multiplexing possibilities. The PEG derivatives of rather hydrophilic molecules such as amino acids and glutathione were successfully retained on a standard C18 reversed-phase column, and their identification was facilitated based on m/z values and retention times using extracted ion chromatograms. The mass increase due to PEG derivatization moved low molecular weight metabolite signals out of the often noisy, low m/z region of the mass spectra, which resulted in enhanced overall sensitivity and selectivity. Furthermore, elution at increased retention times resulted in efficient electrospray ionization due to the higher acetonitrile content in the mobile phase. The method was successfully applied to the quantification of intracellular amino acids and glutathione in a cellular model of human lung epithelium exposed to cigarette smoke-induced oxidative stress. It was shown that the concentration of most amino acids increased upon exposure of A549 cells to gas-phase cigarette smoke with respect to air control and cigarette smoke extract and that free thiol-containing species (e.g., glutathione) decreased although disulfide bond formation was not increased. These labeling reagents should also prove useful for the labeling of peptides and other compounds containing primary amine functionalities.

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