BCA Protein Assay Kit | Boster Immunoleader AR0146 product information

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company name :

Boster Immunoleader

product type :

other

product name :

BCA Protein Assay Kit

catalog :

AR0146

quantity :

1 kit

price :

60 USD

publications citing this reagent :

Huang Y, Wang Y, Li X, Chen Z, Li X, Wang H, et al. Molecular mechanism of ER stress-induced gene expression of tumor necrosis factor-related apoptosis-inducing ligand (TRAIL) in macrophages. FEBS J. 2015;282:2361-78 pubmed publisher
An P, Dang H, Shi X, Ye B, Wu X. "Qufeng Tongluo" acupuncture prevents the progression of glomerulonephritis by decreasing renal sympathetic nerve activity. J Ethnopharmacol. 2014;155:277-84 pubmed publisher
Peng X, Jiang Y. Protective effects of Lactobacillus plantarum NDC 75017 against lipopolysaccharide-induced liver injury in mice. Inflammation. 2014;37:1599-607 pubmed publisher
Liu X, Qian L, Nan H, Cui M, Hao X, Du Y. Function of the transforming growth factor-β1/c-Jun N-terminal kinase signaling pathway in the action of thalidomide on a rat model of pulmonary fibrosis. Exp Ther Med. 2014;7:669-674 pubmed
Cheng C, Huang C, Ma T, Bian E, He Y, Zhang L, et al. SOCS1 hypermethylation mediated by DNMT1 is associated with lipopolysaccharide-induced inflammatory cytokines in macrophages. Toxicol Lett. 2014;225:488-97 pubmed publisher
Cheng G, Zhao Y, Li H, Wu Y, Li X, Han Q, et al. Forsythiaside attenuates lipopolysaccharide-induced inflammatory responses in the bursa of Fabricius of chickens by downregulating the NF-κB signaling pathway. Exp Ther Med. 2014;7:179-184 pubmed
He Y, Sun X, Huang C, Long X, Lin X, Zhang L, et al. MiR-146a regulates IL-6 production in lipopolysaccharide-induced RAW264.7 macrophage cells by inhibiting Notch1. Inflammation. 2014;37:71-82 pubmed publisher
Chen J, Wang J, Yu C, Chen L, Xu P, Yu W. Total flavonoids of Mosla scabra leaves attenuates lipopolysaccharide-induced acute lung injury via down-regulation of inflammatory signaling in mice. J Ethnopharmacol. 2013;148:835-41 pubmed publisher
Ying H, Liu Y, Yu B, Wang Z, Zang J, Yu C. Dietary quercetin ameliorates nonalcoholic steatohepatitis induced by a high-fat diet in gerbils. Food Chem Toxicol. 2013;52:53-60 pubmed publisher
Gui J, Xiong F, Li J, Huang G. Effects of acupuncture on Th1, th2 cytokines in rats of implantation failure. Evid Based Complement Alternat Med. 2012;2012:893023 pubmed

more info or order :

Boster Immunoleader product webpage

product information

Code :

AR0146

Name :

BCA Protein Assay Kit

Size :

1 kit

Price :

60 USD

SubCategory :

Western Blotting Related Reagent

Storage :

BCA Reagent A & B should be stored at 4˚C; Albumin Standard Ampules should be stored at -20˚C.

Indtroduction :

The BCA Protein Assay is a detergent-compatible formulation based on bicinchoninic acid (BCA) for the colorimetric detection and quantization of total protein. This method combines the well-known reduction of Cu+2 to Cu+1 by protein in an alkaline medium (the biuret reaction) with the highly sensitive and selective colorimetric detection of the cuprous cation (Cu+1) using a unique reagent containing bicinchoninic acid. The purple-colored reaction product of this assay is formed by the chelation of two molecules of BCA with one cuprous ion. This water-soluble complex exhibits a strong absorbance at 562 nm that is nearly linear with increasing protein concentrations over a broad working range (20-2,000 ug/ml). The BCA method is not a true end-point method; that is, the final color continues to develop. However, following incubation, the rate of continued color development is sufficiently slow to allow large numbers of samples to be assayed together. The macromolecular structure of protein, the number of peptide bonds and the presence of four particular amino acids (cysteine, cystine, tryptophan and tyrosine) are reported to be responsible for color formation with BCA.2 Studies with di-, tri- and tetrapeptides suggest that the extent of color formation caused by more than the mere sum of individual color producing functional groups. Accordingly, protein concentrations generally are determined and reported with reference to standards of a common protein such as bovine serum albumin (BSA). A series of dilutions of known concentration are prepared from the protein and assayed alongside the unknown before the concentration of each unknown is determined based on the standard curve. If precise quantization of an unknown protein is required, it is advisable to select a protein standard that is similar in quality to the unknown; for example, a bovine gamma globulin (BGG) standard may be used when assaying immunoglobulin samples. Two assay procedures are presented. Of these, the Test Tube Procedure requires a larger volume (0.1 ml) of protein sample; however, because it uses a sample to working reagent ratio of 1:20 (v/v), the effect of interfering substances is minimized.

Protocol :

Preparation of Standards and Working Reagent (required for both assay procedures) A. Preparation of Diluted Albumin (BSA) Standards Use Table 1 as a guide to prepare a set of protein standards. Table 1. Preparation of Diluted Albumin (BSA) Standards 1. BCA Regent A to BCA Regent B ratio = 50:1 (i.e. Add 1ml BCA Reagent B into 50ml BCA Reagent A). 2．Dilution Scheme for Standard Test Tube Protocol and Microplate Procedure (Working Range = 25–2,000ug/ml) (Dilute the lyophilized Albumin Standard Ampules with 0.9% NaCl or PBS to 2,000ug/ml working solution ) Tube Volume of Diluen Volume and Source of BSA Final BSA Concentration A 0ul 600ul 2000ug/ml B 100ul 300ul 1500ug/ml C 300ul 300ul of A dilution 1000ug/ml D 200ul 200ul of B dilution 750ug/ml E 300ul 300ul of C dilution 500ug/ml F 300ul 300ul of E dilution 250ug/ml G 300ul 300ul of F dilution 125ug/ml H 400ul 100ul of G dilution 25ug/ml I 300ul 0ul 0ug/ml（blank） Test Tube Procedure (Sample to WR ratio = 1:20) 1. Pipette 0.1 ml of each standard and unknown sample replicate into an appropriately labeled test tube. 2. Add 2.0 ml of the WR to each tube and mix well. 3. Cover and incubate tubes at selected temperature and time: a. Standard Protocol: 37˚C for 30 minutes (working range = 25-2,000 ug/ml) b. RT Protocol: RT for 2 hours (working range = 25-2,000 ug/ml) c. Enhanced Protocol: 60˚C for 30 minutes (working range = 5-250 ug/ml) Notes: Increasing the incubation time and temperature can increase the net 562 nm absorbance for each test and decreases both the minimum detection level of the reagent and the working range of the protocol. Use a water bath to heat tubes for either Standard (37˚C incubation) or Enhanced (60˚C incubation) Protocol. Using a forced-air incubator can introduce significant error in color development because of uneven heat transfer. 4. Cool all tubes to RT. 5. With the spectrophotometer set to 562 nm, zero the instrument on a cuvette filled only with water. Subsequently, measure the absorbance of all the samples within 10 minutes. Note: Because the BCA Assay does not reach a true end point, color development will continue even after cooling to RT. However, because the rate of color development is low at RT, no significant error will be introduced if the 562 nm absorbance measurements of all tubes are made within 10 minutes of each other. 6. Subtract the average 562 nm absorbance measurement of the Blank standard replicates from the 562 nm absorbance measurement of all other individual standard and unknown sample replicates. 7. Prepare a standard curve by plotting the average Blank-corrected 562 nm measurement for each BSA standard vs. its concentration in ug/ml. Use the standard curve to determine the protein concentration of each unknown sample. Microplate Procedure (Sample to WR ratio = 1:8) 1. Pipette 25 ul of each standard or unknown sample replicate into a microplate well (working range = 25-2,000 ug/ml). Note: If sample size is limited, 10 ul of each unknown sample and standard can be used (sample to WR ratio = 1:20). However, the working range of the assay in this case will be limited to 125-2,000 ug/ml. 2. Add 200 ul of the WR to each well and mix plate thoroughly on a plate shaker for 30 seconds. 3. Cover plate and incubate at 37˚C for 30 minutes. 4. Cool plate to RT. 5. Measure the absorbance at or near 562 nm on a plate reader. Notes: a. Wavelengths from 540-595 nm have been used successfully with this method. b. Because plate readers use a shorter light path length than cuvette spectrophotometers, the Microplate Procedure requires a greater sample to WR ratio to obtain the same sensitivity as the standard Test Tube Procedure. If higher562 nm measurements are desired, increase the incubation time to 2 hours. Troubleshooting 1. When the temperature is law or storage tine is long, sediments may occur. Please mix round or incubate at 37˚C, or microwave for 30 seconds to melt it. If any bacteria contamination is found, please abandon it. 2. If sample contains EDTA. EGTA. DTT. ammonia sulfate or lipid, it will interrupt the result, please try Bradford protein concentration test kit; the detergent at high concentration will interrupt the result, try to remove them by TCA sediments. 3. To get more exact protein concentration result, make sure each SAAG and sample has a second well, try to deal with standard Ampules and sample in a same method( such as use a same dilution and regent). And erytime should make a standard curve. 4. When Regent A mixes with Regent B, few sediments may occur. It will fade away after be mixed thoroughly. 5. 37˚C water bath, incubator, ELISA reader, spectrophotometer which light length is between 540-595nm are required.

Application :

For quantitation of total protein

Number of assays :

50 test tube or 500 micro plate assays

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