CCAT2 Knockout HT-29 Cell Line

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The CCAT2 Knockout HT-29 Cell Line provides a CRISPR/Cas9-edited loss-of-function model of the oncogenic long non-coding RNA CCAT2 in human colorectal adenocarcinoma cells. This engineered cell line enables targeted investigation of CCAT2-dependent signaling in the context of an APC-mutant, TP53-mutant, KRAS-mutant background.

CCAT2 functions by binding TCF7L2 to enhance MYC expression and drive proliferation and invasion, while also acting as a ceRNA for miR-145. The knockout cell line is a valuable tool for colorectal cancer research, Wnt pathway analysis, and drug screening studies.

SKU: ARG0436 Categories: ,

Description

The CCAT2 Knockout HT-29 Cell Line is a genetically engineered human colorectal adenocarcinoma cell model generated by CRISPR/Cas9-mediated disruption of the CCAT2 gene locus. This loss-of-function cell line enables precise investigation of CCAT2-dependent molecular mechanisms in colorectal cancer. Established in the HT-29 epithelial background, the knockout product is supplied as a ready-to-use cell line optimized for downstream assays. The targeted gene ablation is achieved through CRISPR/Cas9 technology, providing a stable and reproducible system for functional genomics studies.

The HT-29 parental cell line was originally derived from a primary colorectal adenocarcinoma of a 44-year-old female and represents a widely utilized model in intestinal cancer research. HT-29 cells harbor well-characterized oncogenic mutations in APC, TP53, and KRAS, resulting in constitutively active Wnt/??-catenin signaling and aberrant cell proliferation. The epithelial morphology and robust in vitro growth characteristics make HT-29 a preferred host for studying colorectal cancer biology, epithelial?Cmesenchymal transition, and therapeutic interventions.

CCAT2 is a long non-coding RNA that functions as a potent oncogene in colorectal cancer. It physically interacts with TCF7L2 to enhance transcriptional activation of the MYC proto-oncogene, driving expression of proliferation and invasion regulators such as CCND1 and MMP7. CCAT2 also acts as a ceRNA, sponging tumor-suppressive miRNAs like miR-145. These activities are integrated into the Wnt/??-catenin pathway, where upstream Wnt ligands (e.g., Wnt3a) through Frizzled/LRP receptors stabilize ??-catenin, which then complexes with TCF7L2 and CCAT2 to activate a pro-tumorigenic transcriptional program.

In HT-29 cells, APC loss-of-function mutations result in constitutive ??-catenin stabilization and persistent TCF/LEF transcriptional activity. CCAT2 knockout therefore disrupts a critical downstream effector of aberrant Wnt signaling, enabling dissection of lncRNA-specific contributions to tumor cell proliferation, survival, and invasiveness. This model is particularly useful for validating CCAT2 as a therapeutic target and for studying lncRNA function in a mutationally defined colorectal cancer background.

Applications include RT-qPCR and Western blot for expression analysis of CCAT2, MYC, CCND1, and ??-catenin; TOP/FOP Flash luciferase assays for TCF/LEF activity; RNA immunoprecipitation for CCAT2-TCF7L2 interaction; proliferation (MTT/CCK-8), colony formation, and Transwell migration/invasion assays; cell cycle analysis by flow cytometry; and in vivo xenograft tumor models. The cell line also supports high-throughput drug screening for Wnt/MYC inhibitors and transcriptomic studies via RNA-seq. For additional information or to inquire about custom gene-edited cell models, please contact Ascent Research.

Additional information

Product Type

Genome-edited Cells

Tissue Source

Large intestine (colon)

Disease

Adenocarcinoma

Size/Quantity

1 million

Shipping info

Cryopreserved in vials and shipped on dry ice

Host Cell

HT-29

Morphology

Epithelial-like

Age

44 years

Sex of Donor

Female

Gene Name

CCAT2

Gene Species

Homo sapiens (Human)

Gene Identifier

NCBI Gene ID 101805488

Temperature

37

Atmosphere

5% CO2

Sterility testing

Daily monitoring confirms that the cells are free from bacterial, yeast, and fungal contamination.

Mycoplasma testing

Negative for mycoplasma through PCR analysis

Pathogens

Cells tested negative for HIV-1, HBV, and HCV.

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