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21019

硫酸铯

Name: 硫酸铯
Brand: SIGALD

puriss. p.a., ≥99.5% (T)

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关于此项目

经验公式（希尔记法）:

Cs₂O₄S

化学文摘社编号:

10294-54-9

分子量:

361.87

UNSPSC Code:

12352300

PubChem Substance ID:

329751899

EC Number:

233-662-6

MDL number:

MFCD00010959

Assay:

≥99.5% (T)

Form:

solid

Solubility:

H₂O: 0.2 g/mL, clear, colorless

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属性

grade

puriss. p.a.

assay

≥99.5% (T)

form

solid

impurities

≤0.001% total nitrogen (N)

mp

1019 °C (lit.)

solubility

H₂O: 0.2 g/mL, clear, colorless

density

4.243 g/mL at 25 °C (lit.)

anion traces

chloride (Cl^-): ≤20 mg/kg

cation traces

Ca: ≤10 mg/kg, Cd: ≤5 mg/kg, Co: ≤5 mg/kg, Cr: ≤5 mg/kg, Cu: ≤5 mg/kg, Fe: ≤5 mg/kg, K: ≤50 mg/kg, Mg: ≤5 mg/kg, Mn: ≤5 mg/kg, Na: ≤50 mg/kg, Ni: ≤5 mg/kg, Pb: ≤5 mg/kg, Zn: ≤5 mg/kg

SMILES string

[Cs+].[Cs+].[O-]S([O-])(=O)=O

InChI

1S/2Cs.H2O4S/c;;1-5(2,3)4/h;;(H2,1,2,3,4)/q2*+1;/p-2

InChI key

FLJPGEWQYJVDPF-UHFFFAOYSA-L

说明

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存储类别

13 - Non Combustible Solids

wgk

WGK 2

flash_point_f

Not applicable

flash_point_c

Not applicable

法规信息

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分析证书(COA)

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5-Fluoro-2'-deoxyuridine incorporation in L1210 DNA.

D W Kufe et al.

The Journal of biological chemistry, 256(17), 8885-8888 (1981-09-10)

We have employed cesium sulfate density gradient centrifugation to separate RNA and DNA of L1210 cells labeled with [3H]fluorodeoxyuridine. We have analyzed nucleotide and nucleoside digests of purified DNA from the [3H]fluorodeoxyuridine-labeled cells and demonstrate by reverse phase and anion

Action of neuropeptide Y on nociceptive transmission in substantia gelatinosa of the adult rat spinal dorsal horn.

A Miyakawa et al.

Neuroscience, 134(2), 595-604 (2005-06-25)

Effects of neuropeptide Y (NPY) on substantia gelatinosa neurons were investigated in adult rat spinal cord slices using blind whole-cell patch-clamp technique. Bath application of NPY (1 microM) induced a membrane hyperpolarization, resulting in a suppression of the dorsal root

An automated method for determining buoyant density of nucleic acids using a preparative ultracentrifuge.

A K Attri et al.

Analytical biochemistry, 159(1), 88-95 (1986-11-15)

We present a technique for analytical buoyant density sedimentation of nucleic acids which is performed in a preparative ultracentrifuge, in contrast to an analytical ultracentrifuge. Following centrifugation in a preparative rotor, small cylindrical quartz tubes are optically scanned; upon completion

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