世界*實(shí)驗(yàn)材料供應(yīng)商 BioCheck正式授權(quán)上海起發(fā)為其中國(guó)代理, BioCheck在一直是行業(yè)的*,一直為廣大科研客戶提供zui為的產(chǎn)品和服務(wù),上海起發(fā)一直秉承為中國(guó)科研客戶帶來(lái)的產(chǎn)品,的服務(wù),簽約 BioCheck就是為了給廣大科研客戶帶來(lái)更加完善的產(chǎn)品和服務(wù),您的滿意將是我們zui大的收獲
BioCheck中國(guó)代理, BioCheck上海代理, BioCheck北京代理,BioCheck廣東代理, BioCheck江蘇代理BioCheck湖北代理,BioCheck天津,BioCheck黑龍江代理,BioCheck內(nèi)蒙古代理,BioCheck吉林代理,BioCheck福建代理, BioCheck江蘇代理, BioCheck浙江代理, BioCheck四川代理
BIOCHECK公司由創(chuàng)始人 Dr. John Chen, Medix創(chuàng)立, 是一家抓也提供腫瘤標(biāo)志物,心肌標(biāo)志物,激素類zui高性價(jià)比的抗體的公司。
簡(jiǎn)要原理
利用競(jìng)爭(zhēng)酶聯(lián)免疫方法,預(yù)先在微孔中包被羊抗兔抗體,實(shí)驗(yàn)時(shí)先后加入氯霉素標(biāo)準(zhǔn)品或待測(cè)樣本,氯霉素酶標(biāo)抗原和兔抗氯霉素抗體。經(jīng)過(guò)室溫溫育,反應(yīng)液中的兔抗氯霉素抗體與微孔板上的羊抗兔抗體結(jié)合,待測(cè)樣品中的抗原與氯霉素酶標(biāo)抗原競(jìng)爭(zhēng)微孔板上的兔抗氯霉素抗體。洗滌后,沒(méi)有與抗
體結(jié)合的待測(cè)樣品中的抗原或酶標(biāo)抗原被洗去,再加入反應(yīng)底物,結(jié)合的酶標(biāo)抗原的酶將底物轉(zhuǎn)化為藍(lán)色產(chǎn)物,加入終止液后顏色由藍(lán)色變?yōu)辄S色。反應(yīng)完成后,樣品中氯霉素含量越多,反應(yīng)呈色就越淺;反之,樣品中氯霉素含量越少,則呈色越深。利用標(biāo)準(zhǔn)曲線可計(jì)算出樣品中氯霉素含量。
技術(shù)參數(shù)
檢測(cè)蜂蜜、蛋類、牛奶、奶粉、水產(chǎn)品、動(dòng)物組織(肌肉、肝臟等)、飼料、血清、血漿及尿液樣本中存在的氯霉素,定量限可達(dá)0.025 ppb。
No. | 樣品 | 檢測(cè)下限 |
1 | 蜂蜜 | 0.02 ppb (0.02 ng/g) |
2 | 蛋類 | 0.02 ppb (0.02 ng/g) |
3 | 牛奶 | 0.002 ppb (0.002 ng/ml) |
4 | 奶粉 | 0.012 ppb (0.012 ng/g) |
5 | 蝦,魚(yú)及肉類 | 0.08 ppb (0.08 ng/g) |
6 | 飼料 | 0.08 ppb (0.08 ng/g) |
7 | 血清/血漿 | 0.02 ppb (0.02 ng/ml) |
8 | 尿液 | 0.04 ppb (0.04 ng/ml) |
交叉反應(yīng)
名稱 | 百分比 |
氯霉素堿 | 0.4% |
甲基氯霉素 | <0.04% |
回收率
No. | 樣品 | 回收率 |
1 | 蜂蜜 | 70% ~ 110% |
2 | 牛奶 | 90% ~ 130% |
3 | 蛋,蝦,魚(yú)及肉類 | 95% ~ 120% |
4 | 飼料 | 95% ~ 120% |
5 | 血清 / 血漿 | 90% ~ 120% |
6 | 尿液 | 100% ~ 130% |
PD-1 ENZYME IMMUNOASSAY TEST KIT
Catalog Number: BC-1301
Enzyme Immunoassay for the Quantitative Determination of PD- 1 Concentration in Human Serum and Plasma
FOR RESEARCH USE ONLY
Not for use in diagnostic procedures
INTRODUCTION
Programmed cell death protein 1, (PD-1, CD279, PDCD1), is a cell surface receptor that is critical for the regulation of T cell inflammatory activity and maintains peripheral tolerance in the immune system (1). With an extracellular IgV domain, a transmembrane domain, and an intracellular tail with two phosphorylation sites (SHP-1 and SHP-2), PD- 1 is able to interact with ligands PD-L1 and PD-L2 to down-regulate the immune system and suppress T cell activity (2). Upon antigen recognition, an activated T cell expresses PD-1 on its surface and produces interferons, which induces expression of PD-L1, thereby promoting apoptosis or cell death. (3) However when hijacked by tumor cells, aberrant expression of PD-1 ligands inhibits immune-modulatory T cell activation, leading to disease progression (4).
Elevated levels of PD-1 in serum and plasma have been associated with rheumatoid arthritis and skin sclerosis (5,6). Also, PD-1 is predominantly expressed by tumor infiltrating T cells(7). Further research implies that using monoclonal antibodies to target the PD-1 immunologic checkpoint has contributed to breakthrough progress in understanding and treating cancers such as melanoma and other various non-small cell lung cancer (4).
PRINCIPLE OF THE ASSAY
The PD-1 ELISA is based on the principle of a solid phase enzyme-linked immunosorbent assay. The assay system utilizes a unique monoclonal antibody pair directed against a distinct antigenic determinant on the PD-1 molecule. One mouse monoclonal anti- PD- 1 antibody is used for solid phase immobilization (on the microtiter wells). Another mouse monoclonal anti-PD-1 antibody conjugated to horseradish peroxidase (HRP) is in the enzyme conjugate solution. The test samples are allowed to react sequentially with the two antibodies, resulting in the PD-1 molecules to be sandwiched between the solid phase and enzyme-linked antibodies. After two separate 60- minute incubation steps at room temperature, the wells are rinsed with Wash Buffer to remove unbound labeled antibodies. TMB Reagent is added and incubated
for 30 minutes under dark conditions, resulting in the development of a blue color. The color development is stopped with the addition of Stop Solution, changing the color to yellow. The concentration of PD-1 is directly proportional to the color intensity of the test samples. Absorbance is measured spectrophotometrically at 450 nm.
REAGENTS AND MATERIALS PROVIDED
Microtiter wells coated with mouse monoclonal anti-PD-1
50 ng/mL PD-1 in phosphate buffer-BSA solution with preservatives
3. Standard and Sample Diluent (30 mL/bottle, 1 bottle)
Contains phosphate buffer-BSA solution with preservatives
Contains mouse monoclonal anti-PD-1 conjugated to horseradish peroxidase
Contains one-step TMB solution
Contains diluted hydrochloric acid (1N HCl)
STORAGE CONDITIONS
REAGENT PREPARATION
ASSAY PROCEDURE
CALCULATION OF RESULTS
data reduction may be employed.
EXAMPLE OF STANDARD CURVE
Results of a typical standard run with absorbency readings at 450 nm shown on the Y axis against PD -1 concentrations shown on the X axis. NOTE: This standard curve is for the purpose of illustration only, and should not be used to calculate unknowns. Each laboratory must generate its own data and standard curve in each experiment.
PD-1 | Absorbance |
(ng/ml) | (450 nm) |
0 | 0.089 |
0.156 | 0.138 |
0.313 | 0.190 |
0.625 | 0.284 |
1.25 | 0.481 |
2.5 | 0.851 |
5 | 1.581 |
10 | 2.776 |
nm | 3 |
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2.5 |
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(450 |
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2 |
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Absorbance | 1.5 |
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1 |
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0.5 |
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0 |
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| 0 | 2 | 4 | 6 | 8 | 10 |
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| PD-1 Conc. (ng/ml) |
|
PERFORMANCE CHARACTERISTICS
The minimum detectable concentration of the PD-1 ELISA assay as measured by 2SD from the mean of a zero standard is estimated to be 0.15 ng/ml.
Within-run precision was determined by replicate determinations of three different samples in one assay. Within-assay variability is shown below:
Sample | 1 | 2 | 3 |
# Replicates | 24 | 24 | 24 |
Mean PD-1 (ng/mL) | 8.4 | 13.2 | 22.9 |
S.D. | 0.6 | 1.0 | 0.9 |
C.V. (%) | 7.0% | 7.2% | 3.8%. |
2
Between-run precision was determined by replicate measurements of three different samples over a series of individually calibrated assays. Between-assay variability is shown below:
Sample | 1 | 2 | 3 |
# Replicates | 20 | 20 | 20 |
Mean PD-1 (ng/mL) | 9.1 | 13.5 | 25.3 |
S.D. | 0.8 | 1.1 | 0.9 |
C.V. (%) | 9.2% | 7.9 | 3.7 |
Samples were spiked with known PD-1 levels and assayed in duplicate. The mean recovery was 105.3%.
PAIR | EXPECTED | OBSERVED | % RECOVERY |
NUMBER | [PD-1] | [PD-1] |
|
| (ng/mL) | (ng/mL) |
|
1 | 8 | 8.8 | 110.0% |
2 | 12.5 | 13.1 | 104.8% |
3 | 25 | 25.3 | 101.2% |
Three samples were serially diluted to determine linearity. The mean recovery was 99.6%.
# | Dilution | Expected | Observed |
|
|
| Conc. (ng/ml) | Conc. (ng/ml) | % Expected |
1. | 1:2 |
| 10.1 | 114.8% |
| 1:4 | 8.8 | 8.8 | N/A |
| 1:8 |
| 7.8 | 88.6% |
|
|
|
| Mean = 101.7% |
|
|
|
|
|
2. | 1:2 |
| 14.5 | 110.6% |
| 1:4 | 13.1 | 13.1 | N/A |
| 1:8 |
| 11.6 | 88.5% |
|
|
|
| Mean = 99.6% |
3. | 1:2 |
| 26.5 | 104.7% |
| 1:4 | 25.3 | 25.3 | N/A |
| 1:8 |
| 23.0 | 90.0% |
Mean = 97.4%
REFERENCES
Transplantation and the American Society of Transplant
Surgeons, 12(10), 2575–2587.
Cancer Epidemiol Biomarkers Prev. December 1 2014 (23) (12) 2965-2970.
soluble programmed death-1 (sPD-1) is associated with disease activity and radiographic progression in early rheumatoid arthritis. Scandinavian Journal of Rheumatology,43(2), 101-108.
部分產(chǎn)品報(bào)價(jià)如下:
貨號(hào) | 品名 | 規(guī)格 | 價(jià)格 | 品牌 |
BC-1009 | AFP EIA Kit | kit | 3980 | BioCheck |
BC-1011 | CEA EIA Kit | kit | 4016 | BioCheck |
BC-1013 | CA 125 EIA Kit | kit | 4970 | BioCheck |
BC-1015 | CA 15-3 EIA Kit | kit | 4970 | BioCheck |
BC-1017 | CA 19-9 EIA Kit | kit | 4970 | BioCheck |
BC-1019 | PSA EIA Kit* | kit | 3962 | BioCheck |
BC-1021 | Free PSA EIA Kit* | kit | 4196 | BioCheck |
BC-1023 | Free b-hCG EIA Kit | kit | 4196 | BioCheck |
BC-1061 | b-2 Microglobulin EIA Kit § | kit | 4250 | BioCheck |
BC-1001 | TSH EIA Kit § | kit | 3800 | BioCheck |
BC-1003 | U-TSH (S-TSH) EIA Kit § | kit | 3800 | BioCheck |
BC-1005 | T3 EIA Kit § | kit | 3656 | BioCheck |
BC-1006 | Free T3 EIA Kit § | kit | 3890 | BioCheck |
BC-1007 | T4 EIA Kit § | kit | 3656 | BioCheck |
BC-1008 | Free T4 EIA Kit | kit | 3890 | BioCheck |
BC-1081 | Rubella IgG EIA Kit* | kit | 4106 | BioCheck |
BC-1083 | Rubella IgM EIA Kit* | kit | 4196 | BioCheck |
BC-1085 | Toxo IgG EIA Kit* | kit | 3980 | BioCheck |
BC-1087 | Toxo IgM EIA Kit* | kit | 4070 | BioCheck |
BC-1089 | CMV IgG EIA Kit* | kit | 3980 | BioCheck |
BC-1091 | CMV IgM EIA Kit* | kit | 4070 | BioCheck |
BC-1093 | HSV I IgG EIA Kit | kit | 3980 | BioCheck |
BC-1095 | HSV I IgM EIA Kit | kit | 4196 | BioCheck |
BC-1097 | HSV II IgG EIA Kit | kit | 3980 | BioCheck |
BC-1099 | HSV II IgM EIA Kit | kit | 4070 | BioCheck |
BC-1051 | H. pylori IgG (Qualitative) EIA Kit | kit | 4016 | BioCheck |
BC-1052 | H. pylori IgG (Quantitative) EIA Kit | kit | 4106 | BioCheck |
BC-1053 | H. pylori IgM (Qualitative) EIA Kit | kit | 4286 | BioCheck |
BC-1027 | hCG EIA Kit § | kit | 3800 | BioCheck |
BC-1029 | FSH EIA Kit § | kit | 3800 | BioCheck |
BC-1031 | LH EIA Kit § | kit | 3800 | BioCheck |
BC-1037 | Prolactin EIA Kit § | kit | 3800 | BioCheck |
BC-1025 | Human Ferritin EIA Kit § | kit | 3800 | BioCheck |
BC-1033 | HGH EIA Kit § | kit | 3800 | BioCheck |
BC-1035 | IgE EIA Kit § | kit | 3800 | BioCheck |
BC-1203 | Adiponectin EIA Kit* | kit | 7580 | BioCheck |
BC-1105 | Troponin I EIA Kit § | kit | 5330 | BioCheck |
BC-1117 | Myoglobin EIA Kit § | kit | 4250 | BioCheck |
BC-1119 | HS-CRP EIA Kit § | kit | 4250 | BioCheck |
BC-1121 | CK-MB EIA Kit* | kit | 6680 | BioCheck |
BC-1129 | MPO EIA Kit* | kit | 8480 | BioCheck |
BC-1111 | Estradiol EIA Kit § | kit | 4250 | BioCheck |
BC-1113 | Progesterone EIA Kit § | kit | 4250 | BioCheck |
BC-1115 | Testosterone EIA Kit § | kit | 4250 | BioCheck |
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