Sunlong Medical™ Human PD-L2 ELISA Kit_ELISA KIT_Sunlong Medical™_SUNLONG BIOTECH CO., LTD-杭州圣隆生物科技有限公司

Sunlong Medical™ Human PD-L2 ELISA Kit

PDCD1LG2 elisa kit | programmed cell death 1 ligand 2 elisa kit | B7 dendritic cell molecule | B7-DC | B7DC | bA574F11.2 | Btdc | butyrophilin B7-DC | CD273 | MGC142238 | MGC142240 | PD-1 ligand 2 | PD-1-ligand 2 | PD-L2 | PDCD1 ligand 2 | PDCD1L2 | PDL2

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$455.2

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NO.:EL0115Hu

Species:Human

Assay range:46.88pg/mL-3000pg/mL

Sensitivity:4.79 pg/mL

Sample Volume:20 μL

Assay type:Sandwich Method

Validity:Two Years
Goods click count：139
Product Spec: 48T48TPlus$398.00 96T96TPlus$569.00
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Details

Cat NO.:
EL0115Hu

Product:
Sunlong Medical™ Human PD-L2 ELISA Kit

Storage
4℃ (unopened) for two years

Shipping Condition
4℃

Sample Type:
Serum | plasma | cell culture supernatant and other biological samples

Spike Recovery Range:
83% - 117%

Mean Spike Recovery:
0.97

CV of Intra plate:
2.3% - 3.9%

CV of Inter plate:
2.5%-4.4%

NCBI_Gene:
80380

UniProtKB:
Q9BQ51

PLATFORM ELISA

PLATE Detachable 96-well plate

SIZE 96T/48T

STORAGE If the reagent kit is unopened, it should be stored at 4℃. However, if it has been opened, the standard solution should be stored at -20℃, while the other components should be stored at 4℃.

DELIVERY 4℃ blue ice transportation

COMPONENTS 96-well polystyrene enzyme-linked immunosorbent assay (ELISA) plate coated with anti-PD-L2 monoclonal antibody
Human PD-L2 freeze-dried standard
Human PD-L2 detect Antibody
Standard Diluent
Assay Buffer(10×)
Substrate TMB
Stop Solution
Washing Buffer(20×)
Sealing Film

ASSAY PRINCIPLE This kit utilizes the double antibody sandwich enzyme-linked immunosorbent assay (ELISA) detection technique.Specific anti-human PD-L2 antibodies are precoated on a high-affinity ELISA plate. Standard samples, test samples, and the detection antibody labeled with horseradish peroxidase are added to the wells of the ELISA plate. After incubation, PD-L2 present in the samples binds to the solid-phase antibodies and the detection antibodies. After washing, a colorimetric substrate, TMB, is added and the plate is incubated in the dark for color development. The intensity of the color reaction is directly proportional to the concentration of PD-L2 in the samples. A stop solution is added to terminate the reaction, and the absorbance value is measured at a wavelength of 450 nm (with a reference wavelength range of 570-630 nm).

Cat NO.:	EL0115Hu
Product:	Sunlong Medical™ Human PD-L2 ELISA Kit
Storage	4℃ (unopened) for two years
Shipping Condition	4℃
Sample Type:	Serum \| plasma \| cell culture supernatant and other biological samples
Spike Recovery Range:	83% - 117%
Mean Spike Recovery:	0.97
CV of Intra plate:	2.3% - 3.9%
CV of Inter plate:	2.5%-4.4%
NCBI_Gene:	80380
UniProtKB:	Q9BQ51

PLATFORM	ELISA
PLATE	Detachable 96-well plate
SIZE	96T/48T
STORAGE	If the reagent kit is unopened, it should be stored at 4℃. However, if it has been opened, the standard solution should be stored at -20℃, while the other components should be stored at 4℃.
DELIVERY	4℃ blue ice transportation
COMPONENTS	96-well polystyrene enzyme-linked immunosorbent assay (ELISA) plate coated with anti-PD-L2 monoclonal antibody Human PD-L2 freeze-dried standard Human PD-L2 detect Antibody Standard Diluent Assay Buffer(10×) Substrate TMB Stop Solution Washing Buffer(20×) Sealing Film
ASSAY PRINCIPLE	This kit utilizes the double antibody sandwich enzyme-linked immunosorbent assay (ELISA) detection technique.Specific anti-human PD-L2 antibodies are precoated on a high-affinity ELISA plate. Standard samples, test samples, and the detection antibody labeled with horseradish peroxidase are added to the wells of the ELISA plate. After incubation, PD-L2 present in the samples binds to the solid-phase antibodies and the detection antibodies. After washing, a colorimetric substrate, TMB, is added and the plate is incubated in the dark for color development. The intensity of the color reaction is directly proportional to the concentration of PD-L2 in the samples. A stop solution is added to terminate the reaction, and the absorbance value is measured at a wavelength of 450 nm (with a reference wavelength range of 570-630 nm).

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