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H_CALCRL RAMP1 Reporter HEK-293 DDX35™ Cell Line
Description
Cat. No: GM-C37743
Product: H_CALCRL RAMP1 Reporter HEK-293 DDX35TM Cell Line


CGRP family receptors are classified into two subtypes: the calcitonin receptor (CALCR, CTR) that binds CT and the calcitonin receptor-like receptor (CRLR, CLR, CALCRL). The CGRP receptor comprises the calcitonin receptor-like receptor, receptor activity-modifying protein 1 (RAMP1), and CGRP receptor component protein (CRCP).

H_CALCRL RAMP1 Reporter HEK-293 DDX35™ Cell Line is a clonal stable HEK-293 cell line constructed using lentiviral technology, constitutive expression of human CALCRL, human RAMP1, along with cAMP signal-dependent expression of a luciferase reporter gene. When α-CGRP/β-CGRP binds to CALCRL/RAMP1, it activates downstream signaling pathways, leading to the expression of luciferase. Antagonists can inhibit this signal transmission. The luciferase activity measurement indicates the activation level of the signaling pathway and can thus be used to evaluate the in vitro effects of drugs related to CALCRL/RAMP1.

H_CALCRL RAMP1 Reporter HEK-293 DDX35™ Cell Line was obtained through extensive monoclonal screening and multiple rounds of monoclonal selection. It possesses high stability, high sensitivity, and high amplification properties, meeting the standards for customers' batch library construction and release experiments.
Data
The passage stability of response to CGRP (Human). The passage 7, 12, 22, 27, 32 and 37 of H_CALCRL RAMP1 Reporter HEK-293 DDX35™ Cell Line (Cat. GM-C37743) at a concentration of 1.5E4 cells/well (96-well format) was stimulated with serial dilutions of CGRP (Human) (phoenixpeptide/015-02) in assay buffer (DMEM+1% FBS+1% P.S) for 7 hours. The firefly luciferase activity was measured using the GMOne-Step Luciferase Reporter Gene Assay Kit (Cat. GM-040503). Data are shown by drug mass concentration.
The passage stability of response to CGRP II (Human). The passage 7, 12, 22, 27, 32 and 37 of H_CALCRL RAMP1 Reporter HEK-293 DDX35™ Cell Line (Cat. GM-C37743) at a concentration of 1.5E4 cells/well (96-well format) was stimulated with serial dilutions of CGRP II(Human) (phoenixpeptide/015-07) in assay buffer (DMEM+1% FBS+1% P.S) for 7 hours. The firefly luciferase activity was measured using the GMOne-Step Luciferase Reporter Gene Assay Kit (Cat. GM-040503). Data are shown by drug mass concentration.
The passage stability of response to CGRP(Human). The passage 8 and 38 of H_CALCRL RAMP1 Reporter HEK-293 DDX35™ Cell Line (Cat. GM-C37743) at a concentration of 1.5E4 cells/well (96-well format) was stimulated with serial dilutions of CGRP(Human) (phoenixpeptide/015-02) in assay buffer (DMEM+1% FBS+1% P.S) for 7 hours, in triplicate. The firefly luciferase activity was measured using the GMOne-Step Luciferase Reporter Gene Assay Kit (Cat. GM-040503). Data are shown by drug mass concentration.
The passage stability of response to CGRP II(Human). The passage 8 and 38 of H_CALCRL RAMP1 Reporter HEK-293 DDX35™ Cell Line (Cat. GM-C26019) at a concentration of 1.5E4 cells/well (96-well format) was stimulated with serial dilutions of CGRP II(Human) (phoenixpeptide/015-07) in assay buffer (DMEM+1% FBS+1% P.S) for 7 hours, in triplicate. The firefly luciferase activity was measured using the GMOne-Step Luciferase Reporter Gene Assay Kit (Cat. GM-040503). Data are shown by drug mass concentration.
Response to CGRP(Human). The H_CALCRL RAMP1 Reporter HEK-293 DDX35™ Cell Line (Cat. GM-C37743) at a concentration of 1.5E4 cells/well (96-well format) was stimulated with serial dilutions of CGRP(Human) (phoenixpeptide/015-02) in assay buffer (DMEM+1% FBS+1% P.S) for 7 hours. The firefly luciferase activity was measured using the GMOne-Step Luciferase Reporter Gene Assay Kit (Cat. GM-040503). The maximum induction fold was approximately [14.6]. Data are shown by drug mass concentration.
Response to CGRP II(Human). The H_CALCRL RAMP1 Reporter HEK-293 DDX35™ Cell Line (Cat. GM-C37743) at a concentration of 1.5E4 cells/well (96-well format) was stimulated with serial dilutions of CGRP II (phoenixpeptide/015-07) in assay buffer (DMEM+1% FBS+1% P.S) for 7 hours. The firefly luciferase activity was measured using the GMOne-Step Luciferase Reporter Gene Assay Kit (Cat. GM-040503). The maximum induction fold was approximately [15.1]. Data are shown by drug mass concentration.
H_CALCRL RAMP1 Reporter HEK-293 DDX35™ Cell Line (Cat. GM-C37743) was determined by flow cytometry using Anti-CALCRL RAMP1 hIgG2 Antibody(Erenumab)(Cat. GM-51996AB).
Specifications
Cat. NoGM-C37743
ProductH_CALCRL RAMP1 Reporter HEK-293 DDX35™ Cell Line
Product Format1 vial of frozen cells
Quantity5E6 Cells per vial,1 mL
Storage ConditionsLiquid nitrogen immediately upon receipt
Recovery MediumDMEM(Gibco)+10% FBS+1% P.S
Growth mediumDMEM(Gibco)+10% FBS+1% P.S+4 μg/mL Blasticidin+400 μg/mL G418+0.75 μg/mL Puromycin
NoteNone
Freezing Medium90% FBS+10% DMSO
Growth propertiesAdherent
Growth Conditions37°C, 5% CO₂
Safety considerationsBiosafety Level 2
Mycoplasma TestingThe cell line has been screened to confirm the absence of Mycoplasma species.
Materials
ReagentOrdering Information
DMEMGibco/C11995500BT
Fetal Bovine SerumCegrogen biotech/A0500-3010
Pen/StrepThermo/15140-122
BlasticidinGenomeditech/GM-040404
G418Genomeditech/GM-040402
PuromycinGenomeditech/GM-040401
CGRP(Human)phoenixpeptide/015-02
CGRP II(Human)phoenixpeptide/015-07
Anti-CALCRL RAMP1 hIgG2 Antibody(Erenumab)Genomeditech/GM-51996AB
GMOne-Step Luciferase Reporter Gene Assay KitGenomeditech/GM-040503
Cell Culture

Cell Recovery

Recovery Medium: DMEM(Gibco)+10% FBS+1% P.S

To insure the highest level of viability, thaw the vial and initiate the culture as soon as possible upon receipt. If upon arrival, continued storage of the frozen culture is necessary, it should be stored in liquid nitrogen vapor phase and not at -70°C. Storage at -70°C will result in loss of viability.

a)       Thaw the vial by gentle agitation in a 37°C water bath. To reduce the possibility of contamination, keep the O-ring and cap out of the water. Thawing should be rapid (approximately 2 - 3 minutes).

b)       Remove the vial from the water bath as soon as the contents are thawed, and decontaminate by dipping in or spraying with 70% ethanol. All of the operations from this point on should be carried out under strict aseptic conditions.

c)       Transfer the vial contents to a centrifuge tube containing 5.0 mL complete culture medium and spin at approximately 176 x g for 5 minutes. Discard supernatant.

d)       Resuspend cell pellet with the recommended recovery medium. And dispense into appropriate culture dishes.

e)       Incubate the culture at 37°C in a suitable incubator. A 5% CO₂ in air atmosphere is recommended if using the medium described on this product sheet.

Cell Freezing

Freezing Medium: 90% FBS+10% DMSO

a)          Centrifuge at 176 x g for 3 minutes to collect cells.

b)         Resuspend the cells in pre-cooled freezing medium and adjust the cell density to 5E6 cells/mL.

c)          Aliquot 1 mL into each vial.

d)         Place the vial in a controlled-rate freezing container and store at -80°C for at least 1 day, then transfer to liquid nitrogen as soon as possible.

Cell passage

Growth medium: DMEM(Gibco)+10% FBS+1% P.S+4 μg/mL Blasticidin+400 μg/mL G418+0.75 μg/mL Puromycin

For the first 1 to 2 passages post-resuscitation, use the recovery medium. Once the cells have stabilized, switch to a growth medium.

a)          Subculturing is necessary when the cell density reaches 80%. It is recommended to perform subculturing at a ratio of 1:3 to 1:4 every 2-3 days. Ensure that the density does not exceed 80%, as overcrowding can lead to reduced viability due to compression.

b)         Remove and discard culture medium.

c)          Briefly rinse the cell layer with PBS to remove all traces of serum that contains trypsin inhibitor.

d)         Add 1.0 mL of 0.25% (w/v) Trypsin-EDTA solution to dish and observe cells under an inverted microscope until cell layer is dispersed (usually within 30 to 60 seconds at 37°C).

e)          Note: To avoid clumping do not agitate the cells by hitting or shaking the flask while waiting for the cells to detach. Cells that are difficult to detach may be placed at 37°C to facilitate dispersal.

f)          Add 2.0 mL of growth medium to mix well and aspirate cells by gently pipetting.

g)         After centrifugation, resuspend the pellet and add appropriate aliquots of the cell suspension to new culture vessels.

h)         Incubate cultures at 37°C.

Subcultivation Ratio: A subcultivation ratio of 1:3 - 1:4 is recommended

Medium Renewal: Every 2 to 3 days

Notes

a)          Upon initial thawing, a higher number of dead cells is observed, which is a normal phenomenon. Significant improvement is seen after adaptation. Once the cells reach a stable state, the number of dead cells decreases after subculturing and the cell growth rate becomes stable.

b)         Ensure that the cell density does not exceed 80%, as overcrowding may lead to reduced viability due to compression.

 

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Current Position:Product Center > Cell lines > GPCR > CALCA(CGRP) > H_CALCRL RAMP1 Reporter HEK-293 DDX35™ Cell Line
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H_CALCRL RAMP1 Reporter HEK-293 DDX35™ Cell Line
Description
Cat. No: GM-C37743
Product: H_CALCRL RAMP1 Reporter HEK-293 DDX35TM Cell Line


CGRP family receptors are classified into two subtypes: the calcitonin receptor (CALCR, CTR) that binds CT and the calcitonin receptor-like receptor (CRLR, CLR, CALCRL). The CGRP receptor comprises the calcitonin receptor-like receptor, receptor activity-modifying protein 1 (RAMP1), and CGRP receptor component protein (CRCP).

H_CALCRL RAMP1 Reporter HEK-293 DDX35™ Cell Line is a clonal stable HEK-293 cell line constructed using lentiviral technology, constitutive expression of human CALCRL, human RAMP1, along with cAMP signal-dependent expression of a luciferase reporter gene. When α-CGRP/β-CGRP binds to CALCRL/RAMP1, it activates downstream signaling pathways, leading to the expression of luciferase. Antagonists can inhibit this signal transmission. The luciferase activity measurement indicates the activation level of the signaling pathway and can thus be used to evaluate the in vitro effects of drugs related to CALCRL/RAMP1.

H_CALCRL RAMP1 Reporter HEK-293 DDX35™ Cell Line was obtained through extensive monoclonal screening and multiple rounds of monoclonal selection. It possesses high stability, high sensitivity, and high amplification properties, meeting the standards for customers' batch library construction and release experiments.
Data
The passage stability of response to CGRP (Human). The passage 7, 12, 22, 27, 32 and 37 of H_CALCRL RAMP1 Reporter HEK-293 DDX35™ Cell Line (Cat. GM-C37743) at a concentration of 1.5E4 cells/well (96-well format) was stimulated with serial dilutions of CGRP (Human) (phoenixpeptide/015-02) in assay buffer (DMEM+1% FBS+1% P.S) for 7 hours. The firefly luciferase activity was measured using the GMOne-Step Luciferase Reporter Gene Assay Kit (Cat. GM-040503). Data are shown by drug mass concentration.
The passage stability of response to CGRP II (Human). The passage 7, 12, 22, 27, 32 and 37 of H_CALCRL RAMP1 Reporter HEK-293 DDX35™ Cell Line (Cat. GM-C37743) at a concentration of 1.5E4 cells/well (96-well format) was stimulated with serial dilutions of CGRP II(Human) (phoenixpeptide/015-07) in assay buffer (DMEM+1% FBS+1% P.S) for 7 hours. The firefly luciferase activity was measured using the GMOne-Step Luciferase Reporter Gene Assay Kit (Cat. GM-040503). Data are shown by drug mass concentration.
The passage stability of response to CGRP(Human). The passage 8 and 38 of H_CALCRL RAMP1 Reporter HEK-293 DDX35™ Cell Line (Cat. GM-C37743) at a concentration of 1.5E4 cells/well (96-well format) was stimulated with serial dilutions of CGRP(Human) (phoenixpeptide/015-02) in assay buffer (DMEM+1% FBS+1% P.S) for 7 hours, in triplicate. The firefly luciferase activity was measured using the GMOne-Step Luciferase Reporter Gene Assay Kit (Cat. GM-040503). Data are shown by drug mass concentration.
The passage stability of response to CGRP II(Human). The passage 8 and 38 of H_CALCRL RAMP1 Reporter HEK-293 DDX35™ Cell Line (Cat. GM-C26019) at a concentration of 1.5E4 cells/well (96-well format) was stimulated with serial dilutions of CGRP II(Human) (phoenixpeptide/015-07) in assay buffer (DMEM+1% FBS+1% P.S) for 7 hours, in triplicate. The firefly luciferase activity was measured using the GMOne-Step Luciferase Reporter Gene Assay Kit (Cat. GM-040503). Data are shown by drug mass concentration.
Response to CGRP(Human). The H_CALCRL RAMP1 Reporter HEK-293 DDX35™ Cell Line (Cat. GM-C37743) at a concentration of 1.5E4 cells/well (96-well format) was stimulated with serial dilutions of CGRP(Human) (phoenixpeptide/015-02) in assay buffer (DMEM+1% FBS+1% P.S) for 7 hours. The firefly luciferase activity was measured using the GMOne-Step Luciferase Reporter Gene Assay Kit (Cat. GM-040503). The maximum induction fold was approximately [14.6]. Data are shown by drug mass concentration.
Response to CGRP II(Human). The H_CALCRL RAMP1 Reporter HEK-293 DDX35™ Cell Line (Cat. GM-C37743) at a concentration of 1.5E4 cells/well (96-well format) was stimulated with serial dilutions of CGRP II (phoenixpeptide/015-07) in assay buffer (DMEM+1% FBS+1% P.S) for 7 hours. The firefly luciferase activity was measured using the GMOne-Step Luciferase Reporter Gene Assay Kit (Cat. GM-040503). The maximum induction fold was approximately [15.1]. Data are shown by drug mass concentration.
H_CALCRL RAMP1 Reporter HEK-293 DDX35™ Cell Line (Cat. GM-C37743) was determined by flow cytometry using Anti-CALCRL RAMP1 hIgG2 Antibody(Erenumab)(Cat. GM-51996AB).
Specifications
Cat. NoGM-C37743
ProductH_CALCRL RAMP1 Reporter HEK-293 DDX35™ Cell Line
Product Format1 vial of frozen cells
Quantity5E6 Cells per vial,1 mL
Storage ConditionsLiquid nitrogen immediately upon receipt
Recovery MediumDMEM(Gibco)+10% FBS+1% P.S
Growth mediumDMEM(Gibco)+10% FBS+1% P.S+4 μg/mL Blasticidin+400 μg/mL G418+0.75 μg/mL Puromycin
NoteNone
Freezing Medium90% FBS+10% DMSO
Growth propertiesAdherent
Growth Conditions37°C, 5% CO₂
Safety considerationsBiosafety Level 2
Mycoplasma TestingThe cell line has been screened to confirm the absence of Mycoplasma species.
Materials
ReagentOrdering Information
DMEMGibco/C11995500BT
Fetal Bovine SerumCegrogen biotech/A0500-3010
Pen/StrepThermo/15140-122
BlasticidinGenomeditech/GM-040404
G418Genomeditech/GM-040402
PuromycinGenomeditech/GM-040401
CGRP(Human)phoenixpeptide/015-02
CGRP II(Human)phoenixpeptide/015-07
Anti-CALCRL RAMP1 hIgG2 Antibody(Erenumab)Genomeditech/GM-51996AB
GMOne-Step Luciferase Reporter Gene Assay KitGenomeditech/GM-040503
Cell Culture

Cell Recovery

Recovery Medium: DMEM(Gibco)+10% FBS+1% P.S

To insure the highest level of viability, thaw the vial and initiate the culture as soon as possible upon receipt. If upon arrival, continued storage of the frozen culture is necessary, it should be stored in liquid nitrogen vapor phase and not at -70°C. Storage at -70°C will result in loss of viability.

a)       Thaw the vial by gentle agitation in a 37°C water bath. To reduce the possibility of contamination, keep the O-ring and cap out of the water. Thawing should be rapid (approximately 2 - 3 minutes).

b)       Remove the vial from the water bath as soon as the contents are thawed, and decontaminate by dipping in or spraying with 70% ethanol. All of the operations from this point on should be carried out under strict aseptic conditions.

c)       Transfer the vial contents to a centrifuge tube containing 5.0 mL complete culture medium and spin at approximately 176 x g for 5 minutes. Discard supernatant.

d)       Resuspend cell pellet with the recommended recovery medium. And dispense into appropriate culture dishes.

e)       Incubate the culture at 37°C in a suitable incubator. A 5% CO₂ in air atmosphere is recommended if using the medium described on this product sheet.

Cell Freezing

Freezing Medium: 90% FBS+10% DMSO

a)          Centrifuge at 176 x g for 3 minutes to collect cells.

b)         Resuspend the cells in pre-cooled freezing medium and adjust the cell density to 5E6 cells/mL.

c)          Aliquot 1 mL into each vial.

d)         Place the vial in a controlled-rate freezing container and store at -80°C for at least 1 day, then transfer to liquid nitrogen as soon as possible.

Cell passage

Growth medium: DMEM(Gibco)+10% FBS+1% P.S+4 μg/mL Blasticidin+400 μg/mL G418+0.75 μg/mL Puromycin

For the first 1 to 2 passages post-resuscitation, use the recovery medium. Once the cells have stabilized, switch to a growth medium.

a)          Subculturing is necessary when the cell density reaches 80%. It is recommended to perform subculturing at a ratio of 1:3 to 1:4 every 2-3 days. Ensure that the density does not exceed 80%, as overcrowding can lead to reduced viability due to compression.

b)         Remove and discard culture medium.

c)          Briefly rinse the cell layer with PBS to remove all traces of serum that contains trypsin inhibitor.

d)         Add 1.0 mL of 0.25% (w/v) Trypsin-EDTA solution to dish and observe cells under an inverted microscope until cell layer is dispersed (usually within 30 to 60 seconds at 37°C).

e)          Note: To avoid clumping do not agitate the cells by hitting or shaking the flask while waiting for the cells to detach. Cells that are difficult to detach may be placed at 37°C to facilitate dispersal.

f)          Add 2.0 mL of growth medium to mix well and aspirate cells by gently pipetting.

g)         After centrifugation, resuspend the pellet and add appropriate aliquots of the cell suspension to new culture vessels.

h)         Incubate cultures at 37°C.

Subcultivation Ratio: A subcultivation ratio of 1:3 - 1:4 is recommended

Medium Renewal: Every 2 to 3 days

Notes

a)          Upon initial thawing, a higher number of dead cells is observed, which is a normal phenomenon. Significant improvement is seen after adaptation. Once the cells reach a stable state, the number of dead cells decreases after subculturing and the cell growth rate becomes stable.

b)         Ensure that the cell density does not exceed 80%, as overcrowding may lead to reduced viability due to compression.

 

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