AKT1 Knockout A-549 Cell Line

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AKT1 Knockout A-549 Cell Line
Cat.No.:

EDC90037

Species:

Human

Cell Name:

A-549

Gene:

AKT1

Gene ID:

207

Size:

1×10⁶cells

AKT1 Knockout Cell Line (A549) is an exclusive upgraded CRISPR/Cas9 system-mediated gene knockout cell, with the advantages of Optimized Strategy Design, Efficient Cell Transfection, High-Performance Cas9 Protein and Hassle-Free Cell Selection.
Cat.No. EDC90037
Product Name AKT1 Knockout A549 Cell Line
Cell Line A-549
Cellosaurus ID CVCL_0023
Cell Line Synonyms A 549, A549, NCI-A549, A549/ATCC, A549 ATCC, A549ATCC, hA549
Gene AKT1
NCBI Gene ID
207
Gene Synonyms AKT|PKB|PKB-ALPHA|PRKBA|RAC|RAC-ALPHA
Summary
This gene encodes one of the three members of the human AKT serine-threonine protein kinase family which are often referred to as protein kinase B alpha, beta, and gamma. These highly similar AKT proteins all have an N-terminal pleckstrin homology domain, a serine/threonine-specific kinase domain and a C-terminal regulatory domain. These proteins are phosphorylated by phosphoinositide 3-kinase (PI3K). AKT/PI3K forms a key component of many signalling pathways that involve the binding of membrane-bound ligands such as receptor tyrosine kinases, G-protein coupled receptors, and integrin-linked kinase. These AKT proteins therefore regulate a wide variety of cellular functions including cell proliferation, survival, metabolism, and angiogenesis in both normal and malignant cells. AKT proteins are recruited to the cell membrane by phosphatidylinositol 3,4,5-trisphosphate (PIP3) after phosphorylation of phosphatidylinositol 4,5-bisphosphate (PIP2) by PI3K. Subsequent phosphorylation of both threonine residue 308 and serine residue 473 is required for full activation of the AKT1 protein encoded by this gene. Phosphorylation of additional residues also occurs, for example, in response to insulin growth factor-1 and epidermal growth factor. Protein phosphatases act as negative regulators of AKT proteins by dephosphorylating AKT or PIP3. The PI3K/AKT signalling pathway is crucial for tumor cell survival. Survival factors can suppress apoptosis in a transcription-independent manner by activating AKT1 which then phosphorylates and inactivates components of the apoptotic machinery. AKT proteins also participate in the mammalian target of rapamycin (mTOR) signalling pathway which controls the assembly of the eukaryotic translation initiation factor 4F (eIF4E) complex and this pathway, in addition to responding to extracellular signals from growth factors and cytokines, is disregulated in many cancers. Mutations in this gene are associated with multiple types of cancer and excessive tissue growth including Proteus syndrome and Cowden syndrome 6, and breast, colorectal, and ovarian cancers. Multiple alternatively spliced transcript variants have been found for this gene. [provided by RefSeq, Jul 2020]
Associated Diseases Non-Small Cell Lung Carcinoma
Morphology Adherent
Passage Ratio 1/5-1/4 ,2days
Complete Culture Medium F-12K + 10% FBS
Freezing Medium 95% Complete culture medium + 5% DMSO
QC Indels validated by Sanger sequencing; sterility confirmed via microbial testing.
* For research use only. Not intended for use in humans or animals, including clinical, therapeutic, or diagnostic purposes.
LociSTR Info (Sample Cell)
Sample Cell Line: A-549		STR Info (Cell bank)
Cell Line: A-549
Allele1Allele2Allele1Allele2
Amelogenin X Y X Y
CSF1PO 10 12 10 12
D2S1338 24 24
D3S1358 16 16
D5S818 11 11
D7S820 8 11 8 11
D8S1179 13 14 13 14
D13S317 11 11
D16S539 11 12 11 12
D18S51 14 17 14 17
D19S433 13 13
D21S11 29 29
FGA 23 23
Penta D 9 9
Penta E 7 11 7 11
TH01 8 9.3 8 9.3
TPOX 8 11 8 11
vWA 14 14
D6S1043 11 13
D12S391 18 18
D2S441 10 13 10 13
* STR authentication data of this cell line matches with that of cell lines sourced from ATCC, DSMZ, JCRB, and RIKEN databases.
Conclusion: The STR identification of this cell is correct.

FAQ

AKT (Protein Kinase B) is a family of three paralogous serine/threonine kinases (AKT1/PKBα, AKT2/PKBβ, AKT3/PKBγ) that are activated downstream of PI3K signaling — PI3K generates PIP3, which recruits AKT to the plasma membrane via its PH domain; AKT is then phosphorylated at T308 (activation loop, by PDK1) and S473 (hydrophobic motif, by mTORC2) for full activation. AKT family members share substantial substrate scope but have distinct tissue expression and functions: AKT1 is broadly expressed and important in cell survival/growth; AKT2 is enriched in insulin-sensitive tissues (liver, muscle, adipose) and central to insulin signaling; AKT3 is enriched in brain and testis with roles in neural development. Substantial paralog redundancy means that single-isoform knockouts often show modest phenotypes — paired and combination knockouts are essential for systematic functional dissection. This AKT1 Knockout in A-549 enables study of AKT1-specific functions — AKT1 is the broadly expressed AKT isoform with critical roles in cell survival, proliferation, growth, and angiogenesis; AKT1 activating mutations (E17K in the PH domain, most common) drive PI3K-AKT pathway hyperactivation and are observed in HR+ breast cancer (~3-5%). Overexpression is useful for studying AKT1 gain-of-function effects (e.g., E17K activating mutation). For AKT-targeted cancer therapy research, the EDITGENE AKT1 Knockout in A-549 is the cornerstone of EDITGENE's complete AKT paralog dissection toolkit in A-549 (single AKT1, single AKT2, double AKT1&AKT2, double AKT1&AKT3, double AKT2&AKT3). Rescue with wild-type, kinase-dead (K179M), E17K activating mutation, or myristoylated constitutively active AKT1 enables comprehensive structure-function studies. The knockout is a critical specificity tool for ⭐⭐ capivasertib (Truqap, FDA-approved 2023 — particularly active in AKT1 E17K-mutated and PIK3CA-mutated cancers), ipatasertib, MK-2206, ARQ-092 in cancer drug development.
Primary applications: • AKT1-specific signaling: AKT1-dependent survival, proliferation, growth analysis. • Cancer mutation rescue: E17K PH domain activating mutation enables HR+ breast cancer modeling. • AKT family paralog dissection: parallel analysis with AKT2 KO and the three double KOs in A-549 (all available) for systematic paralog studies. • Capivasertib specificity: critical genetic control for ⭐⭐ capivasertib (FDA-approved 2023 — particularly active against AKT1 E17K-mutated breast cancer). EDITGENE recommends this AKT1 single KO as the cornerstone of the systematic AKT paralog dissection toolkit for capivasertib-class cancer drug development.
Yes. AKT1 rescue experiments are gold-standard for cancer AKT research: • Construct design: use a codon-modified AKT1 sequence with a small C-terminal tag (FLAG, HA). Preserve PH domain (PIP3 binding), kinase domain (T308 activation site), and C-terminal hydrophobic motif (S473). • Kinase-dead rescue: K179M ATP-binding lysine mutation abolishes catalytic activity. • Cancer mutation rescue: ⭐ E17K PH domain activating mutation (HR+ breast cancer) — gold-standard for capivasertib pharmacology. • Constitutively active rescue: myr-AKT1 constitutive plasma membrane localization. • Functional readout: rescue should restore AKT1-specific cell survival/growth signaling. A-549-specific considerations: • A-549 is a human non-small cell lung carcinoma (NSCLC) cell line widely used for lung cancer drug development. • Lentiviral transduction is supported with moderate efficiency. • A-549's PI3K-AKT pathway activity makes it a relevant context for systematic AKT paralog research.
* Research Use Disclaimer: Content is generated from publicly available research data, bioinformatic resources, and computational analyses for research reference only.

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