Human USP14 Knockout Cell Line-Hela
Cat.No. : CSC-RT0138
Host Cell: Hela Target Gene: USP14
Size: >1x10^6 cells/vial, 1mL Validation: Sequencing
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Cell Line Information
Cell Culture Information
Safety and Packaging
| Cat. No. | CSC-RT0138 |
| Cell Line Information | This cell line is a stable cell line with a homozygous knockout of human USP14 using CRISPR/Cas9. |
| Target Gene | USP14 |
| Gene ID | 9097 |
| Genotype | USP14 (-/-) |
| Host Cell | Hela |
| Cell Type | Epithelial |
| Size | >1x10^6 cells/vial, 1mL |
| Sequencing Result | Allele 1: 8 bp deletion in exon Allele 2: 1 bp deletion in exon |
| Revival | Rapidly thaw cells in a 37°C water bath. Transfer contents into a tube containing pre-warmed media. Centrifuge cells and seed into a 25 cm2 flask containing pre-warmed media. |
| Media Type | Cells were cultured in DMEM supplemented with 10% fetal bovine serum. |
| Growth Properties | Cells are cultured as a monolayer at 37°C in a humidified atmosphere with 5% CO2. Split at 80-90% confluence, approximately 1:4-1:6. |
| Freeze Medium | Complete medium supplemented with 10% (v/v) DMSO |
| Mycoplasma | Negative |
| Format | One frozen vial containing millions of cells |
| Storage | Liquid nitrogen |
| Safety Considerations |
The following safety precautions should be observed. 1. Use pipette aids to prevent ingestion and keep aerosols down to a minimum. 2. No eating, drinking or smoking while handling the stable line. 3. Wash hands after handling the stable line and before leaving the lab. 4. Decontaminate work surface with disinfectant or 70% ethanol before and after working with stable cells. 5. All waste should be considered hazardous. 6. Dispose of all liquid waste after each experiment and treat with bleach. |
| Ship | Dry ice |
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Background
Case Study
Applications
USP14, also known as ubiquitin-specific peptidase 14, is an enzyme that plays a key role in regulating protein degradation within cells. It is part of the ubiquitin-proteasome system (UPS), which maintains cellular homeostasis by degrading misfolded, damaged, or unnecessary proteins. The UPS involves a multistep process in which proteins are initially tagged with ubiquitin molecules to be degraded by the proteasome, a large protein complex with proteolytic activity.
Studies have shown that USP14 is involved in various cellular processes beyond protein degradation. For example, it has been implicated in synaptic function and neurodegenerative diseases. Aberrant activity of USP14 has been linked to diseases such as Alzheimer's and Parkinson's diseases, where misregulation of protein degradation leads to the accumulation of toxic protein aggregates. The role of USP14 in regulating the degradation of key proteins involved in these pathways makes it an important target for therapeutic intervention. In addition, USP14 has been implicated in cancer biology. Many studies have shown that USP14 can regulate the stability of oncoproteins and tumor suppressors. Its dysregulation has been observed in various cancer types, suggesting that inhibition of USP14 may be a viable strategy for cancer therapy.
The ubiquitin-proteasome system (UPS) and autophagy are two major intracellular degradation mechanisms that mediate the turnover of complementary pools of the intracellular proteome. Simultaneous activation of the UPS and autophagy may provide a powerful strategy for the clearance of misfolded proteins. However, it is unclear whether the UPS and autophagy can be controlled by common regulatory mechanisms. K48 deubiquitination of USP14 is known to inhibit the UPS. Here, researchers demonstrate that USP14 regulates autophagy by negatively controlling K63 ubiquitination of Beclin 1. Furthermore, Akt-mediated activation of USP14 by phosphorylation provides a mechanism for Akt to negatively regulate autophagy by promoting K63 deubiquitination. These studies suggest that Akt-regulated USP14 activity regulates proteasomal degradation and autophagy by controlling K48 and K63 ubiquitination, respectively. Thus, regulation of USP14 provides a mechanism for Akt to control both proteasomal and autophagic degradation. Inhibition of USP14 may provide a strategy to promote UPS and autophagy for the development of novel therapeutics for neurodegenerative diseases.
To test whether phosphorylation of USP14 is required for its DUB activity (K63 ubiquitination of Beclin 1), wild-type USP14 or mutant USP14 were stably expressed in Usp14 knockout cells and the effects on Beclin 1 ubiquitination were examined. As shown in Figure 1C, expression of wild-type USP14 or the USP14-DD mutant, but not the USP14-AA mutant, inhibited K63 ubiquitination of Beclin 1. Expression of wild-type USP14 inhibited Beclin 1 ubiquitination in the presence or absence of Myr-Akt expression, whereas expression of the USP14-AA mutant failed to inhibit Beclin 1 ubiquitination even in the presence of activated Akt (Figure 1D), indicating that USP14-regulated deubiquitination of Beclin 1 is dependent on Akt-mediated phosphorylation. Furthermore, even in the presence of the Akt inhibitor MK2206, the USP14-DD mutant was still able to reduce the ubiquitination level of Beclin 1, whereas wild-type USP14 lost its deubiquitination activity on Beclin 1 after Akt inhibition ( Figure 1E ). Taken together, these results suggest that Akt-mediated phosphorylation of USP14 regulates its K63 deubiquitination activity on Beclin 1.
Figure 1. Akt-mediated phosphorylation regulates the activity of USP14 DUB against Beclin 1. (A) H4 cells were serum starved overnight, and lysates were analyzed by immunoprecipitation with anti-Beclin 1, and immune complexes were analyzed by Western blot analysis with anti-ubiquitin K63-specific antibody. (B) H4 cells were infected with Myr-Akt lentiviral vector for 12 h and then serum starved for another 12 h, and lysates were analyzed by immunoprecipitation with anti-Beclin 1, and immune complexes were analyzed by A. (C) Usp14−/− H4 cells were transfected with wild-type USP14 or mutant viruses for 24 h, and lysates were analyzed by immunoprecipitation with anti-Beclin 1, and immune complexes were analyzed by Western blot analysis. (D) Usp14 knockout H4 cells were virally transfected with wild-type USP14 or USP14-AA mutants (with or without Myr-Akt as indicated) for 24 h, lysates were immunoprecipitated with anti-Beclin 1, and immune complexes were analyzed as in C. (E) Usp14 knockout H4 cells were virally transfected with wild-type USP14 or USP14-DD mutants for 18 h and then treated with or without 1 µM MK2206 for 6 h, lysates were immunoprecipitated with anti-Beclin 1, and immune complexes were analyzed as in D. (Xu, Daichao, et al. 2016)
The USP14 gene encodes a deubiquitinating enzyme that is involved in protein degradation by the ubiquitin-proteasome system. By eliminating this gene, the USP14 knockout cell line provides a powerful tool for a variety of research applications:
Protein degradation studies: This cell line can be used to study the role of USP14 in the ubiquitin-proteasome system. Researchers can study how USP14 deficiency affects protein stability and turnover, providing insights into protein homeostasis.
Drug discovery: USP14 is a target for drug development due to its regulatory role in protein degradation. The knockout cell line can be used in high-throughput screening assays to identify potential inhibitors or modulators of USP14 activity.
Cancer research: Given that HeLa cells are derived from cervical carcinoma, the USP14 knockout HeLa cell line can be used to explore the relationship between USP14 and cancer progression, metastasis, and chemotherapy response.
Neurodegenerative disease models: USP14 has been implicated in neurodegenerative diseases such as Alzheimer's and Parkinson's diseases. This cell line can be used to create in vitro models to study pathways involved in these diseases and test therapeutic approaches.
Cellular pathway analysis: By examining the effects of USP14 loss on various cellular pathways, researchers can gain greater insight into its role in cell cycle regulation, apoptosis, and other cellular processes.
Proteomic studies: USP14 knockout cell lines can serve as models for proteomic studies to identify changes in the ubiquitinome and other post-translational modifications that occur in the absence of USP14.
For research use only. Not intended for any clinical use.
