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QIA56  MMP-9 ELISA Kit

Gelatinase B ELISA Kit, 92 kDa Gelatinase ELISA Kit, Matrix Metalloproteinase 9 ELISA Kit

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01 Juni 2012

wird geladen
 
Bestellnummer St./Pkg. Menge Preis
QIA56-1EA  1 ea  wird geladen
Preisänderungen vorbehalten.
A non-isotopic, sandwich ELISA for the in vitro measurement of human MMP-9 in tissue culture supernatant, serum, or plasma.
Produktinformationen
Format 96-well plate
Form 34 or 41 Tests
Detection method Colorimetric
Species reactivity human
Avoid freeze/thaw Ja
Specificity Human pro-MMP-9 protein and MMP-9/TIMP-1 complex
Sensitivity 0.1 ng/ml
Assay range 0.625 - 20 ng/ml
Assay time 3.5 h
Sample type Tissue culture media, serum, plasma
Kit contains 96-Well Coated Plate, MMP-9 Standard, Biotinylated Detector Antibody, 400X Streptavidin Peroxidase Conjugate, Diluent, Substrate, Assay Buffers, Stop Solution, Plate Sealer, and a user protocol.
Declaration Not available for sale in Japan.
Lager- und Versandinformationen

Achtung Gefahrgut:Aufgrund der Natur des in dieser Lieferung enthaltenen Gefahrgutes können zusätzliche Versandkosten für Ihren Auftrag entstehen. Bestimmte Größen können ggf. von den Versandzuschlägen für Gefahrgüter ausgenommen sein. Bitte kontaktieren Sie Ihr lokales Verkaufsbüro für weitere Informationen bzgl. dieser Gebühren.

Lagerkategorie -20°C
Ship Dry Ice Only
Multiple Toxicity Values, refer to MSDS
Sicherheitshinweise
S-Satz S: 26-36/37/39-45



R-Satz R: 23/24/25-35-36-40-43





Daten

The mean signal of each standard run in replicates of four in eight assays using two different lots of plates and two different lots of detector antibody.


The pooled coefficients of variation (according to the formula of Henry et. al., 1974) and between assay coefficients of variation are plotted against MMP-9 concentrations. The pooled data were collected from samples run eight times using two different lots of plates and two different lots of detector antibody in replicates of four on two separate occasions.

The study tested dilution-recovery of ten positive samples. The dilutions were run in the MMP-9 ELISA Kit and the "found" doses were plotted against the "expected" doses to determine linearity of dilution. The slope is not significantly different from one and the intercept is not significantly different from zero. These studies are consistent with the absence of cross-reacting and matrix effects such as pH, salts, and endogenous binders that interfere with the reagents used in the assay. <b>Note:</b> Ca = Cancer; NHS = Normal Human Sera; NHP = Normal Human Plasma; PMA = Phorbol 12-myristate 13-acetate; EGF = Epidermal Growth Factor; AR = Amphiregulin; Both = EGF and AR; A = 2 x 10<sup>6</sup> cells/ml; B = 1.0 x 10<sup>6</sup> cells/ml.

Levels of MMP-9 detected by the ELISA after immunoaffinity extraction of MMP-9 positive samples (PMA treated HT1080 and HL-60 cells) with a MMP-9 antibody that is not used in the ELISA, a TIMP-1 antibody, a TIMP-2 antibody and a TIMP-3 antibody.

APMA promotes the autocatalytic cleavage of the N-terminal propeptide of the latent 92-kDa enzyme to yield the active form of the enzyme. Analysis of the samples by zymography showed both cleavage of the proenzyme by APMA and a good correlation with the levels of the proenzyme determined with the MMP-9 ELISA. Several methods of MMP-9 induction were used to generate positive samples such as treatment with 50 ng/ml amphiregulin (AR), 50 ng/ml epidermal growth factor (EGF), 1 ng/ml transforming growth factor β (TGFβ) and 25 ng/ml phorbol 12-myristate 13-acetate (PMA). Normal human sera (NHS) containing moderate levels of MMP-9 were treated with APMA and analyzed.

© Merck KGaA, Darmstadt, Deutschland, 2012


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