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Purmorphamine

Name: Purmorphamine
Brand: Selleck Chemicals
SKU: S3042
Rating: 5 (36 reviews)

Catalog No.S3042 Synonyms: Shh Signaling Antagonist VI

For research use only.

Purmorphamine (Shh Signaling Antagonist VI), which directly binds and activates Smoothened, blocks BODIPY-cyclopamine binding to Smo with IC50 of ~ 1.5 μM in HEK293T cell and also is an inducer of osteoblast differentiation with EC50 of 1 μM. Purmorphamine can reduce both basal and induced autophagy.

CAS No. 483367-10-8

Selleck's Purmorphamine has been cited by 36 publications

Purity & Quality Control

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Hedgehog/Smoothened Signaling Pathway Map

Biological Activity

Description

Targets

Smoothened ^[1]
(HEK293T cells)

~1.5 μM

In vitro

Purmorphamine activates the Hedgehog pathway by directly binds and activates Smoothened with IC50 of ~ 1.5 μM in compete with cyclopamine, a Smo antagonist. ^[1] Purmorphamine is a potent inducer of osteogenesis in multipotent C3H10T1/2 cells. The EC50 (based on ALP expression) for Purmorphamine is 1 μM in C3H10T1/2 cells. Purmorphamine (1 μM) and BMP-4 (100 ng/mL) together increase ALP activity more than 90-fold in 3T3-L1 cells. ^[2] In contrast to BMP-4, Purmorphamine induces osteogenesis by activating Hedgehog signaling in multipotent mesenchymal progenitor cells. ^[3]

Cell Data

Cell Lines	Assay Type	Concentration	Incubation Time	Formulation	Activity Description	PMID

C3H10T1/2	M2SwNWZ2dmO2aX;uJIF{e2G7		Mn7aOkBl[Xm\|	MWDBZ5Rqfmm2eTDheEBUdW9iaX6gcY92e2ViQ{PINVBVOS9{IHPlcIx{KGG\|c3Xzd4VlKGG\|IHnu[JVkfGmxbjDv[kBk\WyuIHTp[oZmemWwdHnheIlwdiCrboTvJI9{fGWxYnzhd5QhcW6ldXLheIVlKG[xcjC2JIRigXNiYomgZYxs[WyrbnWgdIhwe3CqYYThd4Uh[XO\|YYmsJGVEPTBiPTCwMlgh\|ryPLh?=	M1\xNFxiKHSjcnfleF0oZ2KuYX7rK{BpemWoPTfoeJRxezpxL4D1Zo1m\C6wY3LpMo5tdS6waXiu[493NzJ5NEK5NlU2Lz5{N{SyPVI2PTxxYU6=
Shh Light2	M2fRbmZ2dmO2aX;uJIF{e2G7		NXfQdpREOzBiaILz	MkDzRYN1cX[jdHnvckBw\iCVaHigbY4hdW:3c3WgV4hpKEyrZ3j0NkBk\WyuczDh[pRmeiB\|MDDodpMh[nlibIXjbYZmemG\|ZTDy[ZBwenSncjDn[Y5mKGG\|c3H5MEBGSzVyIE2gNUDPxE1w	MnPGQIEhfGG{Z3X0QUdg[myjbnunJIhz\WZ;J3j0eJB{Qi9xcIXicYVlNm6lYnmucoxuNm6raD7nc5YwOTZ2MEiwPFgoRjF4NEC4NFg5RC:jPh?=
C3H10T1/2	MojYSpVv[3Srb36gZZN{[Xl?			MorITY5lfWO2aX;uJI9nKG:\|dHXv[4Vv\XOrczDpckBud3W\|ZTDDN2gyOFRzL{KgZ4VtdHNiYYPz[ZN{\WRiYYOgbY5lfWO2aX;uJI9nKG:\|dHXvZoxie3Ric4DlZ4lncWNibXHyb4VzKGGua3HsbY5mKHCqb4PwbIF1[XOnIHL5JIludXWwb3\seY9z\XOlZX7j[UBu\XSqb3SsJGVEPTBiPTCxJO69VS5?	M4TFV\|xiKHSjcnfleF0oZ2KuYX7rK{BpemWoPTfoeJRxezpxL4D1Zo1m\C6wY3LpMo5tdS6waXiu[493NzF4NEC4NFA{Lz5zNkSwPFAxOzxxYU6=
HEK293T	Ml7HSpVv[3Srb36gZZN{[Xl?		NH;EboIyKGi{	MmnRTY5pcWKrdHnvckBw\iCET1TJVHku[3mlbH;wZY1qdmViYnnu[Ilv\yC2bzDTcY8h\XiycnXzd4VlKGmwIFjFT\|I6O1RiY3XscJMh[W[2ZYKgNUBpeiCkeTDmcJVwemW\|Y3XuZ4UhdWmlcn;zZ49xgSxiSVO1NEA:KDFwNTFOwG0v	NXL0V3FIRGFidHHy[4V1RSehYnzhcosoKGi{ZX[9K4h1fHC\|Oj:vdJVjdWWmLn7jZokvdmyvLn7pbE5od3ZxMU[0NFgxQDhpPkG2OFA5ODh6PD;hQi=>
Shh Light2	MoHRSpVv[3Srb36gZZN{[Xl?		MYCzNEBpenN?	MVrBZ5RqfmG2aX;uJI9nKFOqaDDpckBud3W\|ZTDTbIghVGmpaISyJINmdGy\|IHHzd4V{e2WmIHHzJIJmfGFvZ3HsZYN1d3OrZHHz[UBi[3Srdnn0fUBi\nSncjCzNEBpenNiYomgcJVkcW[ncnHz[UBz\XCxcoTldkBo\W6nIHHzd4F6KGmwIIDy[ZNmdmOnIH;mJFExOCCwTTCzMYtmfG9vTj3hcYlvd2W2aInsMW4oNWGvaX7vZ4Fxem:7bHTpbJllem:laX7uZY1wgWxiY4njcI9x[W2rbnW=	MWK8ZUB1[XKpZYS9K39jdGGwazegbJJm\j1paIT0dJM7Ny:ydXLt[YQvdmOkaT7ucI0vdmmqLnfvek8yPjRyOEC4PEc,OTZ2MEiwPFg9N2F-
HEK293T	MYjGeY5kfGmxbjDhd5NigQ>?	NFPqOlc2KHWP	NY\YS\|lnPCCqcoO=	MkjmTY5pcWKrdHnvckBw\iCET1TJVHku[3mlbH;wZY1qdmViYnnu[Ilv\yC2bzDTcY8hVi22ZYLtbY5idCCleYP0[Ylv\SCmb33hbY4h\XiycnXzd4VlKGmwIFjFT\|I6O1RiY3XscJMh[XRiNTD1UUBi\nSncjC0JIhzeyCkeTDmcJVwemW\|Y3XuZ4UhdWmlcn;zZ49xgQ>?	NXzLT5hORGFidHHy[4V1RSehYnzhcosoKGi{ZX[9K4h1fHC\|Oj:vdJVjdWWmLn7jZokvdmyvLn7pbE5od3ZxMU[0NFgxQDhpPkG2OFA5ODh6PD;hQi=>
HEK293T	M1z0cWZ2dmO2aX;uJIF{e2G7	NIHjbpc2KHWP	MVi0JIhzew>?	MnznTY5pcWKrdHnvckBw\iCET1TJVHku[3mlbH;wZY1qdmViYnnu[Ilv\yC2bzDTcY8hSy22ZYLtbY5idCCleYTvdIxie22rYzDkc41icW5iZYjwdoV{e2WmIHnuJGhGUzJ7M2SgZ4VtdHNiYYSgOUB2VSCjZoTldkA1KGi{czDifUBndHWxcnXzZ4Vv[2VibXnjdo9{[2:yeR?=	M1uwVlxiKHSjcnfleF0oZ2KuYX7rK{BpemWoPTfoeJRxezpxL4D1Zo1m\C6wY3LpMo5tdS6waXiu[493NzF4NEC4NFg5Lz5zNkSwPFA5QDxxYU6=
SK-N-MC	MnPHdWhVWyCjc4PhfS=>			M{jQZ5FJXFNib3[gdIVlcWG2cnnjJINidmOncjDj[YxtKGyrbnXzJJRwKGmmZX70bYZ6KG23bITpdIxmKG:ycH;yeJVvcXSrZYOg[o9zKGS{dXegdoVxfXKyb4Ppcoc7KFC{aX3hdpkhe2O{ZXXuJIZweiCVSz3OMW1EKGOnbHzz	MUG8ZUB1[XKpZYS9K39jdGGwazegbJJm\j1paIT0dJM7Ny:ydXLt[YQvdmOkaT7ucI0vdmmqLnfvek8zQTR\|NUGzPUc,Ojl2M{WxN\|k9N2F-

Click to View More Cell Line Experimental Data

Assay

Methods	Test Index	PMID

Western blot	Patch1 / Gli1 / LC3 / p62	26609469
Immunofluorescence	SOX18	26588701
Growth inhibition assay	Cell viability	26588701

In vivo

Purmorphamine up-regulates ALP expression in human mesenchymal stem cell-based constructs on rats. ^[4]

Protocol (from reference)

Kinase Assay:^[1]

Binding assay:
Smo binding assays are conducted with BODIPY-cyclopamine and Smo-overexpressing cells as previously described4,5, using CMV promoter-based, SV40 origin-containing expression constructs for Smo-Myc3, the deletion mutant SmoCRD (deletion of amino acids 68 to 182), and SmoCT (deletion of amino acids 556 to 793). HEK 293T cells are grown on poly-D-lysine-treated glass coverslips in 12-well plates until 70% confluency and then transfected with the appropriate expression construct (0.5 g/well) using FuGene 6 according the manufacturer's protocols. Two days after transfection, the HEK 293T cells are incubated with DMEM containing 0.5% bovine calf serum, 5 nM BODIPY-cyclopamine, and varying concentrations of Purmorphamine (0, 1.5, or 5 M) (1 mL/well) for 1 h at 37 ℃. The Smo-overexpressing cells are then washed with 1 × PBS buffer (1 mL/well), mounted with DAPI-containing medium, and visualized using a Leica DM4500B fluorescence microscope. For binding assays using fixed cells, the Smo-overexpressing HEK 293T cells are fixed with 3% paraformaldehyde in 1 × PBS buffer for 10 min at room temperature (1 mL/well), treated with 1 × PBS containing 10 mM glycine and 0.2% sodium azide for 5 min (1 mL/well), washed with 1 × PBS buffer (1 mL/well), and treated with the Purmorphamine-containing media described above for 4 h at room temperature.

Cell Research:^[2]

Cell lines: C3H10T1/2 cell
Concentrations: 0.5-10 μM
Incubation Time: 4 days
Method: C3H10T1/2 cells are expanded in T175 flasks; cells at 13th passage are detached by trypsin/EDTA and diluted in the growth media. The resulting cell suspension is then plated into black clear bottom 384-well plates with 2500 cells/well in 100 µL growth medium using a Multi-drop^TM liquid delivery system. After overnight incubation, cells attached to the bottom of the wells. A stock solution of each Purmorphamine in DMSO (500 nL) is delivered into corresponding well using a Mini Trak^TM multiposition dispenser system to make a final concentration of 5μM of Purmorphamine. Cells are then incubated at 37 ℃ with 5% CO₂ in air atmosphere. After 4 days, the medium is removed and 10 μL of passive lysis buffer is added into each well. After 5 min, 10 μL of alkaline phosphatase substrate solution is added to each well. After incubating 15 min at room temperature, the plates are read on an Acquest high-throughput plate reader following the manufacturer's protocol.

References

[4] Faghihi F, Biomed Pharmacother, 2012, 3322(12).

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Solubility (25°C)

In vitro	DMSO	4 mg/mL warmed (7.68 mM)
	Water	Insoluble
	Ethanol	Insoluble
In vivo	Add solvents to the product individually and in order (Data is from Selleck tests instead of citations): 2% DMSO+30% PEG 300+5% Tween 80+ddH2O For best results, use promptly after mixing. Click to purchase: PEG300 Tween 80	1mg/mL

Chemical Information

Molecular Weight	520.62
Formula	C₃₁H₃₂N₆O₂
CAS No.	483367-10-8
Storage	3 years	-20°C	powder
Storage	2 years	-80°C	in solvent
Smiles	C1CCC(CC1)N2C=NC3=C(N=C(N=C32)OC4=CC=CC5=CC=CC=C54)NC6=CC=C(C=C6)N7CCOCC7

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