Click-IT™ Myristic Acid, Azide (12-Azidododecanoic Acid)
Click-IT™ Myristic Acid, Azide (12-Azidododecanoic Acid)
인용 및 참조 문헌 (4)
Invitrogen™

Click-IT™ Myristic Acid, Azide (12-Azidododecanoic Acid)

Green features
Identify and characterize myristylated proteins with Click-iT® myristic acid, azide using the powerful click chemistry, a simple and robust two-step자세히 알아보기
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카탈로그 번호수량
C102681 mg
카탈로그 번호 C10268
제품 가격(KRW)
778,000
線上優惠
Ends: 31-Dec-2025
972,000
할인액 194,000 (20%)
Each
카트에 추가하기
수량:
1 mg
제품 가격(KRW)
778,000
線上優惠
Ends: 31-Dec-2025
972,000
할인액 194,000 (20%)
Each
카트에 추가하기
Identify and characterize myristylated proteins with Click-iT® myristic acid, azide using the powerful click chemistry, a simple and robust two-step labeling and detection technique. In step one, the azide-containing biomolecule is fed to cells or animals and actively incorporated into proteins. Unlike other labels such as biotin or a fluorescent dye, the azide-tag is small enough that the tagged molecule is an acceptable substrate for the enzymes that incorporate this building block into proteins. Detection utilizes the chemoselective ligation or “click" reaction between and azide and an alkyne where the modified protein is detected with the corresponding alkyne-containing dye or hapten using either the Click-iT® Cell Reaction Buffer Kit or the Click-iT® Protein Buffer Kit. With the Click-iT® Cell Reaction Buffer Kit, cells can be analyzed by fluorescence microscopy, flow cytometry or high-content imaging and analysis (HCS) together with other biomarkers of interest for content and context rich results. With the Click-iT® Protein Reaction Buffer Kit, achieve detection sensitivity in 1-D gels and western blots in the low femtomole range or perform LC-MS⁄MS and MALDI MS analysis.
For Research Use Only. Not for use in diagnostic procedures.
사양
형식Solid
그린 기능Less hazardous
라벨링 방법Metabolic Labeling
제품라인Click-iT, Molecular Probes
제품 유형Myristic Acid
수량1 mg
배송 조건Room Temperature
Labeling TargetProteins, Proteins
라벨 또는 염료Azide
Unit SizeEach
구성 및 보관
Store at ≤-20°C, desiccated and protected from light.

자주 묻는 질문(FAQ)

I am observing no signal or very low signal for my click-labeled samples. What can I do to improve the signal?

The click reaction is only effective when copper is in the appropriate valency. Except for the DIBO alkyne-azide reaction, azides and alkynes will not react with each other without copper. Make sure that the click reaction mixture is used immediately after preparation when the copper (II) concentration is at its highest.
Do not use additive buffer that has turned yellow; it must be colorless to be active.
Cells need to be adequately fixed and permeabilized for the click reagents to have access to intracellular components that have incorporated the click substrate(s).
Some reagents can bind copper and reduce its effective concentration available to catalyze the click reaction. Do not include any metal chelator (e.g., EDTA, EGTA, citrate, etc.) in any buffer or reagent prior to the click reaction. Avoid buffers or reagents that include other metal ions that may be oxidized or reduced. It may be help to include extra wash steps on the cell or tissue sample before performing the click reaction.
You can repeat the click reaction with fresh reagents to try to improve signal. Increasing the click reaction time longer than 30 minutes will not improve a low signal. Performing a second, 30 minute incubation with fresh click reaction reagents is more effective at improving labeling.
Low signal can also be due to low incorporation of EdU, EU, or other click substrates. Other click substrates (e.g., AHA, HPG, palmitic acid, azide, etc.) incorporated into cellular components may have been lost if not adequately cross-linked in place or if the wrong fixative was used. For click substrates that are incorporated into the membrane or lipids, you should avoid the use of alcohol or acetone fixatives and permeabilizing agents.
The incorporated click substrate must be accessible at the time of the click reaction; labeling of incorporated amino acid analogs may be lower in native proteins relative to denatured proteins.
You may need to optimize the metabolic labeling conditions including analog incubation time or concentration. Cells that are healthy, not too high of a passage number and not too crowded may incorporate the analog better. You may create a positive control by including extra doses of the click substrate during multiple time points during an incubation time that spans or closely spans the doubling time of the cell type of interest.

Find additional tips, troubleshooting help, and resources within our Cell Analysis Support Center.

인용 및 참조 문헌 (4)

인용 및 참조 문헌
Abstract
Chemical probes for the rapid detection of Fatty-acylated proteins in Mammalian cells.
Authors:Hang HC, Geutjes EJ, Grotenbreg G, Pollington AM, Bijlmakers MJ, Ploegh HL,
Journal:J Am Chem Soc
PubMed ID:17305342
'New tools are needed to further our understanding of protein fatty acylation. Here we demonstrate that omega-azido fatty acids can be efficiently metabolized by mammalian cells and serve as selective probes to rapidly visualize N-myristoylation and S-acylation, respectively. In addition to the more sensitive detection of fatty-acylated proteins with these ... More
Dynamic monitoring of newly synthesized proteomes: up-regulation of myristoylated protein kinase A during butyric acid induced apoptosis.
Authors:Liu K, Yang PY, Na Z, Yao SQ,
Journal:Angew Chem Int Ed Engl
PubMed ID:21678537
Doubly charged: A double metabolic incorporation approach capable of proteome-wide profiling of post-translational modification dynamics on newly synthesized proteins has been developed (see scheme; blue box: methionine surrogate, orange diamond: PTM probe). This strategy reveals for the first time that up-regulation of myristoylated PKA protein is necessary for the occurrence ... More
Lipid raft-dependent endocytosis of close homolog of adhesion molecule L1 (CHL1) promotes neuritogenesis.
Authors:Tian N, Leshchyns'ka I, Welch JH, Diakowski W, Yang H, Schachner M, Sytnyk V,
Journal:J Biol Chem
PubMed ID:23144456
CHL1 plays a dual role by either promoting or inhibiting neuritogenesis. We report here that neuritogenesis-promoting ligand-dependent cell surface clustering of CHL1 induces palmitoylation and lipid raft-dependent endocytosis of CHL1. We identify ßII spectrin as a binding partner of CHL1, and we show that partial disruption of the complex between ... More
Robust fluorescent detection of protein fatty-acylation with chemical reporters.
Authors:Charron G, Zhang MM, Yount JS, Wilson J, Raghavan AS, Shamir E, Hang HC,
Journal:J Am Chem Soc
PubMed ID:19281244
Fatty-acylation of proteins in eukaryotes is associated with many fundamental cellular processes but has been challenging to study due to limited tools for rapid and robust detection of protein fatty-acylation in cells. The development of azido-fatty acids enabled the nonradioactive detection of fatty-acylated proteins in mammalian cells using the Staudinger ... More