FCCP

別名: Trifluoromethoxy carbonylcyanide phenylhydrazone, Carbonyl cyanide 4-(trifluoromethoxy)phenylhydrazone 中文名稱：碳酰氰-4-三氟甲氧基苯腙

目錄號：S8276 Purity: 99.99%

FCCP (Trifluoromethoxy carbonylcyanide phenylhydrazone, Carbonyl cyanide 4-(trifluoromethoxy)phenylhydrazone)在線粒體中是一種有效的氧化磷酸化的解偶聯(lián)劑，通過轉(zhuǎn)運質(zhì)子破壞ATP的合成。

FCCP Chemical Structure

CAS: 370-86-5

規(guī)格	價格	庫存
10mg	794.76	現(xiàn)貨
50mg	2841.98	現(xiàn)貨
200mg	6527.44	現(xiàn)貨
1g	16298.98	現(xiàn)貨
更大包裝有超大折扣
400-668-6834 info@selleck.cn

產(chǎn)品質(zhì)控

批次：純度： 99.99%

99.99

FCCP相關(guān)產(chǎn)品

相關(guān)產(chǎn)品	IACS-010759 (IACS-10759) Gboxin VLX600 S-Gboxin	點擊展開
相關(guān)化合物庫	自噬化合物庫凋亡分子化合物庫鐵死亡化合物庫細(xì)胞焦亡化合物庫線粒體靶向化合物庫	點擊展開

細(xì)胞實驗數(shù)據(jù)示例

細(xì)胞系	實驗類型	給藥濃度	孵育時間	活性描述	文獻(xiàn)信息
T47D	Function assay	0.3 uM	15 mins	Decrease in mitochondrial membrane potential in human T47D cells 0.3 uM after 15 mins by TMRM assay	20929261
T47D	Function assay	3 uM	15 to 20 mins	Decrease in mitochondrial membrane potential in human T47D cells at 3 uM after 15 to 20 mins by TMRM assay	22938093
SH-SY5Y	Function assay	10 uM	5 mins	Inhibition of SOC in human SH-SY5Y cells assessed as reduction in thapsigargin-induced Ca2+ influx at 10 uM pre-incubated for 5 mins with 0.2 uM CsA followed by compound addition by FURA-2AM dye based fluorescence assay	25265024
SH-SY5Y	Function assay	10 uM	10 mins	Induction of mitochondrial membrane potential loss in human SH-SY5Y cells at 10 uM incubated for 10 mins in presence of 0.2 uM CsA by TMRE dye based assay	25265024
T47D	Function assay	0.3 uM	3 to 12 mins	Increase in oxygen consumption rate of mitochondrial state 4 respiration in human T47D cells assessed as reinitiation of oligomycin-stalled cellular respiration at 0.3 uM incubated for 3 to 12 mins by Clark-type oxygen electrode assay	26637046
T47D	Function assay	0.3 uM	30 mins	Effect on mitochondrial membrane potential in human T47D cells at 0.3 uM after 30 mins by TMRM dye based fluorescence microscopy	26637046
HCT116	Function assay	2 uM	30 mins	Induction of AMPK phosphorylation at Thr-172 residue in human HCT116 cells at 2 uM after 30 mins in glucose supplemented media by immunoblot method	28233680
HCT116	Function assay	2 uM	30 mins	Induction of AMPK phosphorylation at Thr-172 residue in human HCT116 cells at 2 uM after 30 mins in absence of glucose by immunoblot method	28233680
KOPN8	Function assay	10 uM	0.3 hrs	Induction of mitochondrial membrane potential loss in human KOPN8 cells at 10 uM after 0.3 hrs by TMRM staining based flow cytometric analysis	31084028
T47D	Function assay	1 to 10 uM		Inhibition of HIF1-mediated induction of secreted VEGF level in 1, 10-phenanthroline-stimulated human T47D cells at 1 to 10 uM by ELISA	20929261
MDA-MB-231	Cytotoxicity assay	1 uM		Cytotoxicity against human MDA-MB-231 cells assessed as inhibition of cell proliferation/viability at 1 uM	23245650
MDA-MB-231	Cytotoxicity assay	0.1 to 3 uM		Cytotoxicity against human MDA-MB-231 cells assessed as inhibition of cell proliferation/viability at 0.1 to 3 uM in presence of 0.1 uM rotenone mitochondrial electron transport inhibitor	23245650
MDA-MB-231	Function assay	0.3 uM		Stimulation of oligomycin-induced state 4 respiration in human MDA-MB-231 cells at 0.3 uM	23245650
T47D	Function assay	0.1 to 3 uM		Effect on cellular respiration in human T47D cells assessed as increase in oxygen consumption at 0.1 to 3 uM	22938093
T47D	Function assay	10 to 30 uM		Stimulation of state 4 cellular respiration in human T47D cells at 10 to 30 uM in presence of oligomycin	22938093
T47D	Function assay	0.3 to 1 uM		Stimulation of state 4 cellular respiration in human T47D cells at 0.3 to 1 uM in presence of oligomycin	22938093
Hep3B	Function assay	10 uM		Stimulation of state 4 cellular respiration in human Hep3B cells at 10 uM in presence of oligomycin	22938093
Hep3B	Function assay	1 uM		Stimulation of state 4 cellular respiration in human Hep3B cells at 1 uM in presence of oligomycin	22938093
TA3/Ha	Function assay	6 uM		Induction of NAD(P)H oxidation in mouse TA3/Ha cells assessed as reduction of NAD(P)H/NAD(P)+ ratio at 6 uM by spectrofluorometer analysis	24568614
T47D	Function assay	0.3 uM		Increase in oxygen consumption rate in digitonin permeabilized human T47D cells assessed as reinitiation of sodium azide-stalled cellular respiration at 0.3 uM by oxytherm Clark-type electrode assay in presence of ascorbate	26637046
DLD1	Function assay	1 uM		Induction of mitochondrial dysfunction in human DLD1 cells assessed as reduction in mitochondrial ATP production at 1 uM by Seahorse XF real-time assay	31774672
DLD1	Function assay	1 uM		Induction of mitochondrial dysfunction in human DLD1 cells assessed as increase in glycolytic ATP production at 1 uM by Seahorse XF real-time assay	31774672
LS174T	Function assay	1 uM		Induction of mitochondrial dysfunction in human LS174T cells assessed as reduction in mitochondrial ATP production at 1 uM by Seahorse XF real-time assay	31774672
LS174T	Function assay	1 uM		Induction of mitochondrial dysfunction in human LS174T cells assessed as increase in glycolytic ATP production at 1 uM by Seahorse XF real-time assay	31774672
DLD1	Function assay	1 uM		Uncoupling of mitochondrial oxidative phosphorylation in human DLD1 cells at 1 uM in presence of oligomycin A by seahorse XFe96 analyser based assay	31774672
DLD1	Function assay	1 uM		Uncoupling of mitochondrial oxidative phosphorylation in human DLD1 cells assessed as increase in oxygen consumption rate at 1 uM in presence of oligomycin A by seahorse XFe96 analyser based assay	31774672
HEK293	Function assay	1 to 3 uM		Inhibition of LiCl-activated Wnt signaling in HEK293 cells at 1 to 3 uM by TOPFlash reporter gene assay	31774672
T47D	Function assay			Inhibition of hypoxia-induced HIF1 activation in human T47D cells by HRE3-TK-luciferase reporter gene assay, IC50=0.51μM	20929261
T47D	Function assay			Inhibition of 1, 10-phenanthroline-induced HIF1 activation in human T47D cells by HRE3-TK-luciferase reporter gene assay, IC50=0.31μM	20929261
HepG2	Function assay			Luciferase/luciferin-expressing antifolate-resistant parasites were used to infect a culture of HepG2 cells that were pre-incubated with compounds. Infected hepatocytes emit light due to the luciferase reaction. Assay results are presented as the percent , IC50=0.245μM	ChEMBL
點擊查看更多細(xì)胞系數(shù)據(jù)

生物活性

產(chǎn)品描述

靶點

OXPHOS ^[2]

ATP synthase ^[2]

體外研究(In Vitro)
體外研究活性	在體外實驗中，F(xiàn)CCP的處理能誘導(dǎo)細(xì)胞內(nèi)Ca2+迅速升至2倍，同時抑制蛋白合成速率。對蛋白翻譯速率的抑制作用與eIF2α的磷酸化增加以及依賴雙鏈RNA的蛋白激酶活性增加有關(guān)^[1]。 FCCP還可輕微地減少ATP以及活性氧水平，提高線粒體基因如Tfam和COXIV的表達(dá)，誘導(dǎo)老鼠造血干細(xì)胞的靜態(tài)形態(tài)特征以及抑制TGF-β的信號轉(zhuǎn)導(dǎo)^[2]。
細(xì)胞實驗	細(xì)胞系	PC12細(xì)胞
	濃度	30 μM
	孵育時間	30 min, 1h, 2h
	方法	用直徑為24-mm的多孔板，加入含0.175 Ci/mmol的[3H]methionine的新鮮培養(yǎng)液，37℃孵育30分鐘。在不同的時間段對PC12細(xì)胞處理以FCCP，測定蛋白質(zhì)合成速率。

體內(nèi)研究(In Vivo)
體內(nèi)研究活性	FCCP的處理在8細(xì)胞期的小鼠胚胎中可顯著降低線粒體膜電位、ATP的生成以及囊胚中細(xì)胞內(nèi)細(xì)胞團的數(shù)量，對胚泡發(fā)育沒有影響。在胚胎線粒體功能受到干擾的同時，在胚胎植入后，雌性后代的出生體重下降，抑制持續(xù)到斷奶階段。盡管FCCP處理過的雄性小鼠也和雌性小鼠一樣，葡萄糖耐受量降低。但是它們的胰島素敏感度和肥胖度在4-14周內(nèi)無變化。在預(yù)壓胚中，線粒體功能降低，然后減少ATP的輸出，將影響其后代表型^[3]。

參考文獻(xiàn)
[1] Mu?oz F, et al. FEBS Lett. 2001, 492(1-2):156-159. [2] Guimar?es EL, et al. BMC Gastroenterol. 2012, 12:68. [3] Zander-Fox DL, et al. Biol Reprod. 2015, 92(5):124. [4] Cheng M, et al. Int J Mol Sci. 2022 Jan 25;23(3):1320. + 展開

參考文獻(xiàn)

[1] Mu?oz F, et al. FEBS Lett. 2001, 492(1-2):156-159.
[2] Guimar?es EL, et al. BMC Gastroenterol. 2012, 12:68.
[3] Zander-Fox DL, et al. Biol Reprod. 2015, 92(5):124.

[4] Cheng M, et al. Int J Mol Sci. 2022 Jan 25;23(3):1320.

+ 展開

化學(xué)信息&溶解度

分子量	254.17	分子式	C₁₀H₅F₃N₄O
CAS號	370-86-5	SDF	Download FCCP SDF
Smiles	C1=CC(=CC=C1NN=C(C#N)C#N)OC(F)(F)F
儲存條件(自收到貨起)	3年-20°C粉狀	儲備液保存和期限建議分裝儲備液，避免反復(fù)凍融！	1年-80°C溶于溶劑
儲存條件(自收到貨起)	3年-20°C粉狀	儲備液保存和期限建議分裝儲備液，避免反復(fù)凍融！	1個月-20°C溶于溶劑

體外溶解度
批次：

DMSO : 6 mg/mL ( (23.6 mM) ；DMSO吸濕會降低化合物溶解度，請使用新開封DMSO)

Water : Insoluble

Ethanol : Insoluble

DMSO : 51 mg/mL ( (200.65 mM) ；DMSO吸濕會降低化合物溶解度，請使用新開封DMSO)

Ethanol : 51 mg/mL (200.65 mM)

Water : Insoluble

DMSO : 51 mg/mL ( (200.65 mM) ；DMSO吸濕會降低化合物溶解度，請使用新開封DMSO)

Ethanol : 51 mg/mL (200.65 mM)

Water : Insoluble

DMSO : 50 mg/mL ( (196.71 mM) ；DMSO吸濕會降低化合物溶解度，請使用新開封DMSO)

Ethanol : 50 mg/mL (196.71 mM)

Water : Insoluble

摩爾濃度計算器

體內(nèi)溶解度
批次：

現(xiàn)配現(xiàn)用，請按從左到右的順序依次添加，澄清后再加入下一溶劑

動物體內(nèi)配方計算器

實驗計算

摩爾濃度計算器

質(zhì)量	濃度	體積	分子量
=	×	×

稀釋計算器分子量計算器

動物體內(nèi)配方計算器（澄清溶液）

第一步：請輸入基本實驗信息（考慮到實驗過程中的損耗，建議多配一只動物的藥量）

給藥劑量 mg/kg 動物平均體重 g 每只動物給藥體積 μL 動物數(shù)量只

第二步：請輸入動物體內(nèi)配方組成（配方適用于不溶于水的藥物；不同批次藥物配方比例不同，請聯(lián)系Selleck為您提供正確的澄清溶液配方）

% DMSO + % + % Tween 80 + % ddH2O

%DMSO+ %

計算結(jié)果：

工作液濃度： mg/ml；

DMSO母液配制方法： mg 藥物溶于μL DMSO溶液（母液濃度mg/mL，注：如該濃度超過該批次藥物DMSO溶解度，請先聯(lián)系Selleck）；

體內(nèi)配方配制方法：取μL DMSO母液，加入μL PEG300，混勻澄清后加入μL Tween 80，混勻澄清后加入μL ddH₂O，混勻澄清。

體內(nèi)配方配制方法：取μL DMSO母液，加入μL Corn oil，混勻澄清。

注意：1. 首先保證母液是澄清的；
2.一定要按照順序依次將溶劑加入，進(jìn)行下一步操作之前必須保證上一步操作得到的是澄清的溶液，可采用渦旋、超聲或水浴加熱等物理方法助溶。

技術(shù)支持

在訂購、運輸、儲存和使用我們的產(chǎn)品的任何階段，您遇到的任何問題，均可以通過撥打我們的熱線電話400-668-6834，或者技術(shù)支持郵箱tech@selleck.cn，直接聯(lián)系到我們。我們會在24小時內(nèi)盡快聯(lián)系您。

操作手冊

如果有其他問題，請給我們留言。

* 必填項

C1=C0/X	C1:	LOG(C1):
C2=C1/X	C2:	LOG(C2):
C3=C2/X	C3:	LOG(C3):
C4=C3/X	C4:	LOG(C4):
C5=C4/X	C5:	LOG(C5):
C6=C5/X	C6:	LOG(C6):
C7=C6/X	C7:	LOG(C7):
C8=C7/X	C8:	LOG(C8):

成人免费xx,国产又黄又湿又刺激不卡网站,成人性视频app菠萝网站,色天天天天

FCCP

產(chǎn)品質(zhì)控

FCCP相關(guān)產(chǎn)品

細(xì)胞實驗數(shù)據(jù)示例

生物活性

化學(xué)信息&溶解度

實驗計算

技術(shù)支持