Idelalisib (CAL-101, GS-1101)

Catalog No.S2226

Molecular Weight(MW): 415.42

Idelalisib (CAL-101, GS-1101) is a selective p110δ inhibitor with IC50 of 2.5 nM in cell-free assays; shown to have 40- to 300-fold greater selectivity for p110δ than p110α/β/γ, and 400- to 4000-fold more selectivity to p110δ than C2β, hVPS34, DNA-PK and mTOR.

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10mM/1mL In DMSO	USD 156	In stock
10mg	USD 120	In stock
50mg	USD 470	In stock
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Cited by 29 Publications

4 Customer Reviews

Invasive migration of RA FLS was analyzed through growth factor–reduced Matrigel-coated transwell inserts in the presence or absence of 1 µM INK007, 5 µM CAL-101, or 0.3 µM IPI-145, or 0.3 µM GDC-0941 inhibitors or DMSO. Cells were allowed to invade through Matrigel toward PDGF-BB (25 ng/ml) containing media for 24 h and were fixed and stained with Hemacolor staining kit.

J Immunol, 2014, 192(5): 2063-70 . Idelalisib (CAL-101, GS-1101) purchased from Selleck.

293T cells were transfected with HA-tagged Fbxo45. At 48 h after transfection, cells were treated with AKT inhibitor (CAL-101; 10 uM, 4 h), cell extracts from the cytoplasm or nuclei were subjected to IP with anti-HA resin followed by western blot analysis with indicated antibodies.

Cell Death Differ 2014 21(10), 1535-45. Idelalisib (CAL-101, GS-1101) purchased from Selleck.
Isoform-selective PI3K inhibitors blocked PI3K signaling in corresponding Rh30-Myr-p110 cells. Rh30-Myr-p110s cells were cultured in serum-free medium for 12 h, and then exposed to CAL-101 at indicated concentrations for additional 1 h. The cells were collected to detect the level of phosphorylated and total Akt. β-Actin was served as loading control.

Acta Pharmacol Sin 2013 34(9),1201-7. Idelalisib (CAL-101, GS-1101) purchased from Selleck.

After starved in serum-free medium for 24 h,A549 cells incubated with the indicated concentrations of CAL-101 for 3 h,followed by 20-minute stimolation of 100ng/ml EGF.

Dr. Zhang of Tianjin Medical University. Idelalisib (CAL-101, GS-1101) purchased from Selleck.

Purity & Quality Control

Choose Selective PI3K Inhibitors

Biological Activity

Description

Targets

p110δ ^[1] (Cell-free assay)	p110γ ^[1] (Cell-free assay)	p110β ^[1] (Cell-free assay)	p110α ^[1] (Cell-free assay)	hVps34 ^[1] (Cell-free assay)	View More
2.5 nM	89 nM	565 nM	820 nM	978 nM	View More

In vitro

CAL-101 is not sensitive to other PI3K class I subunits including p110α, p110β, and p110γ. CAL-101 specifically blocks FcϵR1 p110δ-mediated CD63 expression with an EC50 of 8 nM in primary basophil. CAL-101 exhibits greater activity in B-cell acute lymphoblastic leukemia (B-ALL) and chronic lymphocytic leukemia (CLL) cells compared with acute myeloid leukemia (AML) and myeloproliferative neoplasm (MPN) cells. CAL-101 produces the reduction in pAktS473, pAktT308, and the downstream target S6 in SU-DHL-5, KARPAS-422 and CCRF-SB cells with EC50 of 0.1 to 1.0 μM. ^[1] CAL-101 induces selective cytotoxicity in CLL cells independent of IgVH mutational status or interphase cytogenetics, primarily through a caspase-dependent mechanism. CAL-101 induces cytotoxicity preferentially to CLL cells compared with normal B cells, without producing cytotoxicity in other hematopoietic cells, compared to LY294002. CAL-101 lacks direct cytotoxic potential to T cells and nature killer (NK) cells. CAL-101 can inhibit production of inflammatory cytokines, such as IL-6, IL-10, TNF-α, and IFN-γ, and activation-induced cytokines, such as CD40L. CAL-101 also antagonizes CD40L-mediated CLL cell survival. ^[2] CAL-101 induces an accumulation of cells in G1 and a decrease in the S-phase population in L1236 and L591 cells, which indicates CAL-101 as a novel strategy for the treatment of hodgkin lymphoma (HL). ^[3]

Cell Data

Cell Lines	Assay Type	Concentration	Incubation Time	Formulation	Activity Description	PMID
MEC1	MXPHdo94fGhiSX7obYJqfGmxbjDBd5NigQ>?			MWLEUXNQ	NIHETnJKSzVyPUKwMlQh\|ryP	MVWyOVk6QTN3Mh?=
CLL PBMCs	M4e0Smdzd3e2aDDJcohq[mm2aX;uJGF{e2G7			Ml22SG1UVw>?	MVrJR\|UxRTJwOTDuUS=>	M4TKU\|I2QTF5Mk[3
U266	NGLhdJFIem:5dHigTY5pcWKrdHnvckBCe3OjeR?=	M3LUOlQxKM7:TR?=	MmW3OFghcA>?		M{DUbVc6NjVnIHnubIljcXSrb36gdoF1\Q>?	MmTyNlU{Ozl\|M{K=
K562	NXLTUpRtTnWwY4Tpc44hSXO\|YYm=	MXuxJO69VQ>?	M2rDS\|MhcA>?		NHL1S5pKdmirYnn0bY9vKG:oIFHreEBxcG:\|cHjvdplt[XSrb36=	M1;DUVI2ODF2N{e1
K562	NHj0c41HfW6ldHnvckBCe3OjeR?=	MoLhNUDPxE1?	MUKzJIg>		MUnJcohq[mm2aX;uJI9nKFB5MGO2T{BxcG:\|cHjvdplt[XSrb36=	Ml7ZNlUxOTR5N{W=
K562	MorxSpVv[3Srb36gRZN{[Xl?	MW[xJO69VQ>?	NEP0[mg{KGh?		MVXJcohq[mm2aX;uJI9nKEeVS{OgdIhwe3Cqb4L5cIF1cW:w	NYHtfno{OjVyMUS3O\|U>
K562	NUDUS2lxT3Kxd4ToJGlvcGmkaYTpc44hSXO\|YYm=	M4\GRVEh\|ryP	NHvMeJY4OiCq		M4DvZ2lvcGmkaYTpc44hd2ZicILvcIln\XKjdHnvci=>	NH3xXYozPTBzNEe3OS=>
Primary AML cell	MmPuSpVv[3Srb36gRZN{[Xl?	NGi2[3MyKM7:TR?=	NYnuOFFUOyCq		MoCwTY5pcWKrdHnvckBw\iCDa4SgdIhwe3Cqb4L5cIF1cW:w	MXeyOVAyPDd5NR?=
Primary AML cell	NVTTU3ZOTnWwY4Tpc44hSXO\|YYm=	NW\MOW57OSEQvF2=	NHXXfFc{KGh?		MYHJcohq[mm2aX;uJI9nKFB5MGO2T{BxcG:\|cHjvdplt[XSrb36=	MX:yOVAyPDd5NR?=
Primary AML cell	NHvjbIhHfW6ldHnvckBCe3OjeR?=	NF;ZdZoyKM7:TR?=	MWCzJIg>		MonkTY5pcWKrdHnvckBw\iCJU1uzJJBpd3OyaH;yfYxifGmxbh?=	MknGNlUxOTR5N{W=
Primary AML cell	NGHp[lFIem:5dHigTY5pcWKrdHnvckBCe3OjeR?=	NXXMc3VCOSEQvF2=	M3[0SlMhcA>?		NXfGcmdWW3WycILld5Nqd25ib3[gdnJPSSC\|eX70bIV{cXN?	M3q4dFI2ODF2N{e1
Microglia	MVHGeY5kfGmxbjDBd5NigQ>?	M2XXcFUh\|ryP	MXexNEBp	NWPUOXRyTE2VTx?=	MVHE[YNz\WG\|ZTDv[kBVVk[jIIPlZ5JmfGmxbjDmdo9uKEySUz3zeIlufWyjdHXkJEBxOTFyzsTEPVExSS:GOUGwRUBucWO{b3fsbYE>	NWfrXYxVOjR4MkW2PFQ>
Primary CLL cell	M2rSdGZ2dmO2aX;uJGF{e2G7	NFXPWpUyKM7:TR?=	NWrhUJc2OTVibXnu	NWXTVFZOTE2VTx?=	M{ewb2Jtd2OtczDCR3IucW6mdXPl[EBNS1BzIIPldolv\S13IHHjeIl3[XSrb36=	NYT2UJROOjRyMEmyN\|M>
JEKO-1	NFLxXZlHfW6ldHnvckBCe3OjeR?=	MoKwNUDPxE1?	NVr4VWc1PzJiaB?=		NF[5NJZKdmirYnn0bY9vKG:oIFHreEBxcG:\|cHjvdplt[XSrb36gbY4hUWePLYP0bY12dGG2ZXSgTmVMVy1z	MonDNlM{PDF3NEG=
Granta-519	NFPkNlRHfW6ldHnvckBCe3OjeR?=	MorpNUDPxE1?	NIm4epczKGh?		MW\Jcohq[mm2aX;uJI9nKEGtdDj0N\|A5MSCyaH;zdIhwenmuYYTpc44>	MmnVNlM{PDF3NEG=
Granta-519	NXewTXFQTnWwY4Tpc44hSXO\|YYm=	M{\LOVEh\|ryP	M{TIRlIhcA>?		MXTJcohq[mm2aX;uJI9nKEGtdDjzOFc{MSCyaH;zdIhwenmuYYTpc44>	NG\wS4gzOzN2MUW0NS=>
JEKO-1	NEK5NmFIem:5dHigTY5pcWKrdHnvckBCe3OjeR?=	NYLNUZI5OTBizszN	NFPDSFc4OiCq		MoHITY5pcWKrdHnvckBw\iCycn;sbYZmemG2aX;uJJNtcWeqdHz5	MWiyN\|M1OTV2MR?=
JEKO-1	NYjueHBGT3Kxd4ToJGlvcGmkaYTpc44hSXO\|YYm=	NUewU3ZsPSEQvF2=	MXS3NkBp		M2HCfIRw\XNibn;0JIlv\HWlZTDj[YxtKGO7Y3zlJIFzemW\|dDDvdkBieG:ydH;zbZM>	M3z0SlI{Pjd4MkKw
MAVER-1	Mn7IS5Jwf3SqIFnubIljcXSrb36gRZN{[Xl?	NILzU3Y2KM7:TR?=	MX:3NkBp		NULTZZc5\G:nczDuc5QhcW6mdXPlJINmdGxiY4njcIUh[XK{ZYP0JI9zKGGyb4D0c5Nqew>?	MYiyN\|Y4PjJ{MB?=
MINO	MnHpS5Jwf3SqIFnubIljcXSrb36gRZN{[Xl?	NY\h[mEzPSEQvF2=	NH7uSlg4OiCq		MXLkc4V{KG6xdDDpcoR2[2ViY3XscEBkgWOuZTDhdpJme3Rib4KgZZBweHSxc3nz	NXvzXmNtOjN4N{[yNlA>
SP53	NF;lOFNIem:5dHigTY5pcWKrdHnvckBCe3OjeR?=	NGLIOYYxNjFizszN	MUK3NkBp		M1rPZ4Rw\XNibn;0JIlv\HWlZTDj[YxtKGO7Y3zlJIFzemW\|dDDvdkBieG:ydH;zbZM>	NIqxSoIzOzZ5NkKyNC=>
HH	NXnDU5FWT3Kxd4ToJGlvcGmkaYTpc44hSXO\|YYm=	NECzW\|MyOCEQvF2=	MY[3NkBp	M4G0TWROW09?	NIe1S45KdmS3Y4Tpc44hd2ZiYYDvdJRwe2m\|IIPsbYdpfGy7	MViyNlgxOTl3OR?=
Myla	MVPHdo94fGhiSX7obYJqfGmxbjDBd5NigQ>?	MYOxNEDPxE1?	NWjOc5ZqPzJiaB?=	MkXMSG1UVw>?	NYfQXWRi\G:nczDuc5QhcW6mdXPlJIFxd3C2b4Ppdy=>	NFnBSJIzOjhyMUm1PS=>
SR786	MkDHS5Jwf3SqIFnubIljcXSrb36gRZN{[Xl?	NIXibIUyOCEQvF2=	M{ewVVczKGh?	MnL6SG1UVw>?	MYTkc4V{KG6xdDDpcoR2[2ViYYDvdJRwe2m\|	Mn;kNlI5ODF7NUm=
HuT78	MnLDS5Jwf3SqIFnubIljcXSrb36gRZN{[Xl?	MoHGNVAh\|ryP	NHH3UWc4OiCq	MXLEUXNQ	M{jvUIRw\XNibn;0JIlv\HWlZTDhdI9xfG:\|aYO=	NFLlbpMzOjhyMUm1PS=>
MJ	MYTHdo94fGhiSX7obYJqfGmxbjDBd5NigQ>?	MmXpNVAh\|ryP	NHz5Ulg4OiCq	NWXMXYhqTE2VTx?=	M4[3fIRw\XNibn;0JIlv\HWlZTDhdI9xfG:\|aYO=	MYiyNlgxOTl3OR?=
DERL7	NGfFVFJIem:5dHigTY5pcWKrdHnvckBCe3OjeR?=	M4LrdlExKM7:TR?=	NXLBdHMyPzJiaB?=	MYLEUXNQ	NH\GOGdld2W\|IH7veEBqdmS3Y3WgZZBweHSxc3nz	M1\qe\|IzQDBzOUW5
L1236	MWfGeY5kfGmxbjDBd5NigQ>?	NEXiU\|AyOCEQvF2=	NVPLb2RKOiCq		M2DOOWlvcGmkaYTpc44hd2ZiQXv0JJBpd3OyaH;yfYxifGmxbh?=	MVqyNlIyODh5Nx?=
L428	NVfi[VhzTnWwY4Tpc44hSXO\|YYm=	NGPH[WsyOCEQvF2=	NWS5eJozOiCq		MojYTY5pcWKrdHnvckBw\iCDa4SgdIhwe3Cqb4L5cIF1cW:w	NYTWVI9LOjJ{MUC4O\|c>
L591	NVP2cGRPTnWwY4Tpc44hSXO\|YYm=	MVGxNEDPxE1?	MX6yJIg>		NFzub4ZKdmirYnn0bY9vKG:oIFHreEBxcG:\|cHjvdplt[XSrb36=	MWCyNlIyODh5Nx?=
KMH-2	M3;hdmZ2dmO2aX;uJGF{e2G7	NHrxWHgyOCEQvF2=	MXWyJIg>		NHTHWJFKdmirYnn0bY9vKG:oIFHreEBxcG:\|cHjvdplt[XSrb36=	NIj3T3ozOjJzMEi3Oy=>
L1236	MV;GeY5kfGmxbjDBd5NigQ>?	NFXlN3g2KM7:TR?=	MX[yOEBp		NX7ndFFlSmyxY3vzJJNm[3KndHnvckBw\iC2aHWgR2NNPQ>?	MonaNlIzOTB6N{e=
L591	MXzGeY5kfGmxbjDBd5NigQ>?	NWTsfng2PSEQvF2=	NV3OepU3OjRiaB?=		MWrCcI9kc3Nic3XjdoV1cW:wIH;mJJRp\SCFQ1y1	MUmyNlIyODh5Nx?=
L1236	MofURZBweHSxc3nzJGF{e2G7	M3SxW\|Uh\|ryP	M2nhOFI1KGh?		MkfUTY5lfWO2aX;uJI9nKGGyb4D0c5Nqew>?	NEHhOmgzOjJzMEi3Oy=>
L591	MYPBdI9xfG:\|aYOgRZN{[Xl?	MlOwOUDPxE1?	MVmyOEBp		MlLJTY5lfWO2aX;uJI9nKGGyb4D0c5Nqew>?	MViyNlIyODh5Nx?=
U-87MG	MnLiSpVv[3Srb36gRZN{[Xl?	MoLTNVAxKG6P	Mn\ZNlQhcA>?	NYPtbVV6TE2VTx?=	M{XBXmlvcGmkaYTpc44hd2ZiIHPlcIwhdWmpcnH0bY9v	MVKyNlA4QTZyOR?=
SW1783	M1nTcWZ2dmO2aX;uJGF{e2G7	NVrlZ4NTOTByIH7N	M2q0OFI1KGh?	NGfoZ2xFVVOR	MYfJcohq[mm2aX;uJI9nKCClZXzsJI1q\3KjdHnvci=>	M4O0V\|IzODd7NkC5
U-87MG	MWHGeY5kfGmxbjDBd5NigQ>?	MWG1JO69VQ>?	NX3WWnA1OjRiaB?=	MnLOSG1UVw>?	NVrC[YR6UW6qaXLpeIlwdiCxZjDBb5QheGixc4Doc5J6dGG2aX;uJJN2[nO2YX70bYFtdHl?	NUjFVoJEOjJyN{m2NFk>
SW1783	NXv4e2xVTnWwY4Tpc44hSXO\|YYm=	MnryOUDPxE1?	Mm[2NlQhcA>?	M{L6PWROW09?	NFO0Zm1KdmirYnn0bY9vKG:oIFHreEBxcG:\|cHjvdplt[XSrb36gd5Vje3SjboTpZYxtgQ>?	MUeyNlA4QTZyOR?=
U-373MG	NY\WVWpbTnWwY4Tpc44hSXO\|YYm=	NVTESlRbPSEQvF2=	MnWzNlQhcA>?	M4q5eGROW09?	MnPiTY5pcWKrdHnvckBw\iCDa4SgdIhwe3Cqb4L5cIF1cW:wIIP1ZpN1[W62aXHscJk>	M4fGcVIzODd7NkC5
SK-MG3	NWrFd4FOTnWwY4Tpc44hSXO\|YYm=	MYS1JO69VQ>?	M4npS\|I1KGh?	MknnSG1UVw>?	M1XhfmlvcGmkaYTpc44hd2ZiQXv0JJBpd3OyaH;yfYxifGmxbjDzeYJ{fGGwdHnhcIx6	M1vDPFIzODd7NkC5
SU-DHL-5	NF;XOItHfW6ldHnvckBCe3OjeR?=	MUCxJO69VQ>?	MXyyOEBp	NXrtS2tITE2VTx?=	NYj0[mZDUW6mdXP0bY9vKG:oIHHwc5B1d3Orcx?=	M2H6N\|IxQTV7NkC2
WSU-NHL	M1LCWGZ2dmO2aX;uJGF{e2G7	M1rrbFEh\|ryP	M3XNdlI1KGh?	NHqxTHVFVVOR	NHvyNmNKdmS3Y4Tpc44hd2ZiYYDvdJRwe2m\|	M1HTUVIxQTV7NkC2
CCRF-SB	NYrwUYFwTnWwY4Tpc44hSXO\|YYm=	NH7jXIEyKM7:TR?=	MV:yOEBp	MlLUSG1UVw>?	M{TZcmlv\HWldHnvckBw\iCjcH;weI9{cXN?	NGOy[IYzODl3OU[wOi=>
INA-6	NFXz[o9HfW6ldHnvckBCe3OjeR?=	NWrS[3NWPSEQvF2=	M4TYVFYhcA>?		M1qz[WlvcGmkaYTpc44hd2ZiUFmzT{9Cc3RiYX7kJGVTUyCyYYToe4F6	NESwZnMzODVyNUG1PC=>
LB	M4THOmZ2dmO2aX;uJGF{e2G7	MYC1JO69VQ>?	Mkf3OkBp		NHXRSVVKdmirYnn0bY9vKG:oIGDJOGswSWu2IHHu[EBGWkticHH0bJdigQ>?	NF;PU3AzODVyNUG1PC=>

... Click to View More Cell Line Experimental Data

Protocol

Kinase Assay:^[2]	+ Expand PI3K assay: PI3K assay is preformed on whole-cell lysates from CLL or normal B cells. A PI3K ELISA assay is performed. Briefly, whole-cell extracts are added to a mixture of PI(4,5)P2 substrate and reaction buffer containing adenosine triphosphate (ATP) and allowed to incubate at room temperature. The reaction is stopped by adding PI(3,4,5)P3 detector mixed with EDTA (ethylenediaminetetraacetic acid) and allowed to incubate at room temperature for 1 hour. After this time, the mixture is transferred from each well to a PI3K ELISA plate and allowed to incubate 1 hour. Plates are washed and then incubated with secondary detector for 30 minutes. Plates are washed again, and 3,3′,5,5′-tetramethylbenzidine solution is added for 5 minutes at which time H2SO4 is added to stop all reactions. Plates are read at 450 nm on a Labsystems 96-well plate reader.
Cell Research:^[2]	+ Expand Cell lines: CLL B cells or healthy volunteer T cells or NK cells Concentrations: 0.01-100 μM Incubation Time: 48 hours Method: MTT assays are performed to determine cytotoxicity. 1 × 10⁵ cells are incubated with CAL-101. MTT reagent is then added, and plates are incubated for an additional 20 hours before washing with protamine sulfate in phosphate-buffered saline. DMSO is added, and absorbance is measured by spectrophotometry at 540 nm in a Labsystems plate reader. Cell viability is also measured at various time points with the use of annexin/PI flow cytometry. Data are analyzed. At least 104 cells are counted for each sample. Results are expressed as the percentage of total positive cells over untreated control. Experiments examining caspase-dependent apoptosis included the addition of 100 μM Z-VAD. Experiments examining survival signals include the addition of 1 μg/mL CD40L, 800 U/mL IL-4, 50 ng/mL BAFF, 20 ng/mL TNF-α, or coculturing on fibronectin or stromal (HS-5 cell line) coated plates. Stromal coculture is done by plating a 75-cm² flask (80%-100% confluent) per 6-well plate 24 hours before the addition of CLL cells. (Only for Reference)

Kinase Assay:^[2]

+ Expand

PI3K assay:

PI3K assay is preformed on whole-cell lysates from CLL or normal B cells. A PI3K ELISA assay is performed. Briefly, whole-cell extracts are added to a mixture of PI(4,5)P2 substrate and reaction buffer containing adenosine triphosphate (ATP) and allowed to incubate at room temperature. The reaction is stopped by adding PI(3,4,5)P3 detector mixed with EDTA (ethylenediaminetetraacetic acid) and allowed to incubate at room temperature for 1 hour. After this time, the mixture is transferred from each well to a PI3K ELISA plate and allowed to incubate 1 hour. Plates are washed and then incubated with secondary detector for 30 minutes. Plates are washed again, and 3,3′,5,5′-tetramethylbenzidine solution is added for 5 minutes at which time H2SO4 is added to stop all reactions. Plates are read at 450 nm on a Labsystems 96-well plate reader.

Cell Research:^[2]

+ Expand

Cell lines: CLL B cells or healthy volunteer T cells or NK cells
Concentrations: 0.01-100 μM
Incubation Time: 48 hours
Method: MTT assays are performed to determine cytotoxicity. 1 × 10⁵ cells are incubated with CAL-101. MTT reagent is then added, and plates are incubated for an additional 20 hours before washing with protamine sulfate in phosphate-buffered saline. DMSO is added, and absorbance is measured by spectrophotometry at 540 nm in a Labsystems plate reader. Cell viability is also measured at various time points with the use of annexin/PI flow cytometry. Data are analyzed. At least 104 cells are counted for each sample. Results are expressed as the percentage of total positive cells over untreated control. Experiments examining caspase-dependent apoptosis included the addition of 100 μM Z-VAD. Experiments examining survival signals include the addition of 1 μg/mL CD40L, 800 U/mL IL-4, 50 ng/mL BAFF, 20 ng/mL TNF-α, or coculturing on fibronectin or stromal (HS-5 cell line) coated plates. Stromal coculture is done by plating a 75-cm² flask (80%-100% confluent) per 6-well plate 24 hours before the addition of CLL cells.
(Only for Reference)

References

Solubility (25°C)

In vitro	DMSO	83 mg/mL warmed (199.79 mM)
	Ethanol	23 mg/mL (55.36 mM)
	Water	Insoluble
In vivo	Add solvents individually and in order: 30% PEG 400 (dissolve first)+0.5% Tween 80+5% Propylene glycol	30mg/mL

* Please note that Selleck tests the solubility of all compounds in-house, and the actual solubility may differ slightly from published values. This is normal and is due to slight batch-to-batch variations.

Chemical Information Download Idelalisib (CAL-101, GS-1101) SDF

Molecular Weight	415.42
Formula	C₂₂H₁₈FN₇O
CAS No.	870281-82-6
Storage	3 years -20°C powder
Synonyms	N/A

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Clinical Trial Information (data from http://clinicaltrials.gov, updated on 2017-02-16)

NCT Number	Recruitment	Conditions	Sponsor/Collaborators	Start Date	Phases
NCT02457598	Recruiting	B-cell Malignancies	Gilead Sciences	June 30, 2015	Phase 1
NCT02962401	Not yet recruiting	Waldenstrom Macroglobulinemia	French Innovative Leukemia Organisation	January 2017	Phase 2
NCT02928510	Not yet recruiting	Absence of Signs or Symptoms\|B-Cell Non-Hodgkin Lymphoma\|Digestive System Signs and Symptoms\|Indolent Adult Non-Hodgkin Lymphoma\|Recurrent B-Cell Non-Hodgkin Lymphoma\|Recurrent Chronic Lymphocytic Leukemia\|Recurrent Indolent Adult Non-Hodgkin Lymphoma\|Recurrent Small Lymphocytic Lymphoma	Jonsson Comprehensive Cancer Center\|Gilead Sciences\|National Cancer Institute (NCI)	January 2017	--
NCT02968563	Recruiting	Chronic Lymphocytic Leukemia	Gilead Sciences\|German CLL Study Group	December 2016	Phase 2
NCT02639910	Recruiting	Leukemia, Lymphocytic, Chronic, B-Cell\|Chronic Lymphocytic Leukemia\|Small Lymphocytic Lymphoma	MorphoSys AG	November 2016	Phase 2
NCT02970318	Recruiting	Chronic Lymphocytic Leukemia	Acerta Pharma BV	September 2016	Phase 3

Tech Support

Answers to questions you may have can be found in the inhibitor handling instructions. Topics include how to prepare stock solutions, how to store inhibitors, and issues that need special attention for cell-based assays and animal experiments.

Handling Instructions

Tel: +1-832-582-8158 Ext:3

If you have any other enquiries, please leave a message.

Frequently Asked Questions

Question 1:
What is the recommended dose of CAL-101 and the route of administration for mouse studies?
Answer:
According to the following paper, S2226 can be used by I.V. administration at the concentration of 40 mg/kg. http://www.ncbi.nlm.nih.gov.ezproxy.liv.ac.uk/pubmed/?term=PI3K%CE%B4+inhibition+reduces+TNF+secretion+and+neuroinflammation+in+a+mouse+cerebral+stroke+model

PI3K Signaling Pathway Map

PI3K Inhibitors with Unique Features

Pan PI3K Inhibitor

LY294002 Pan-PI3Kα/δ/β inhibitor, IC50=0.5 μM/0.57 μM/0.97 μM.
Most Potent PI3K Inhibitor

Duvelisib (IPI-145, INK1197) PI3K δ, IC50=1 nM.
PI3K Inhibitor in Clinical Trial

Hexestrol Phase II for Advanced Breast Cancer.
Newest PI3K Inhibitor

GSK2636771 Potent, orally bioavailable, PI3Kβ-selective inhibitor, sensitive to PTEN null cell lines.

Related PI3K Products

Taselisib (GDC 0032) ^New

Taselisib (GDC 0032) is a potent, next-generation β isoform-sparing PI3K inhibitor targeting PI3Kα/δ/γ with K_i of 0.29 nM/0.12 nM/0.97nM, >10 fold selective over PI3Kβ.

Features:A beta isoform-sparing PI3K inhibitor.
Pilaralisib (XL147) ^New

Pilaralisib (XL147) is a selective and reversible class I PI3K inhibitor for PI3Kα/δ/γ with IC50 of 39 nM/36 nM/23 nM in cell-free assays, less potent to PI3Kβ. Phase 1/2.
GNE-317 ^New

GNE-317 is a potent, brain-penetrant PI3K inhibitor.
LY294002

LY294002 is the first synthetic molecule known to inhibit PI3Kα/δ/β with IC50 of 0.5 μM/0.57 μM/0.97 μM in cell-free assays, respectively; more stable in solution than Wortmannin, and also blocks autophagosome formation.
3-Methyladenine (3-MA)

3-Methyladenine (3-MA) is a selective PI3K inhibitor for Vps34 and PI3Kγ with IC50 of 25 μM and 60 μM in HeLa cells; blocks class I PI3K consistently, whereas suppression of class III PI3K is transient, and also blocks autophagosome formation.
Wortmannin

Wortmannin is the first described PI3K inhibitor with IC50 of 3 nM in a cell-free assay, with little selectivity within the PI3K family. Also blocks autophagosome formation and potently inhibits DNA-PK/ATM with IC50 of 16 nM and 150 nM in cell-free assays.
Dactolisib (BEZ235, NVP-BEZ235)

Dactolisib (BEZ235, NVP-BEZ235) is a dual ATP-competitive PI3K and mTOR inhibitor for p110α/γ/δ/β and mTOR(p70S6K) with IC50 of 4 nM /5 nM /7 nM /75 nM /6 nM in cell-free assays, respectively. Inhibits ATR with IC50 of 21 nM in 3T3^TopBP1-ER cell.
Buparlisib (BKM120, NVP-BKM120)

Buparlisib (BKM120, NVP-BKM120) is a selective PI3K inhibitor of p110α/β/δ/γ with IC50 of 52 nM/166 nM/116 nM/262 nM in cell-free assays, respectively. Reduced potency against VPS34, mTOR, DNAPK, with little activity to PI4Kβ. Phase 2.
Pictilisib (GDC-0941)

Pictilisib (GDC-0941) is a potent inhibitor of PI3Kα/δ with IC50 of 3 nM in cell-free assays, with modest selectivity against p110β (11-fold) and p110γ (25-fold). Phase 2.
Alpelisib (BYL719)

Alpelisib (BYL719) is a potent and selective PI3Kα inhibitor with IC50 of 5 nM in a cell-free assay, and minimal effect on PI3Kβ/γ/δ. Phase 2.

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