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Genetically Modifying CAR T Cells Using a CRISPR-Cas9 System

作者：

简介：

Overview

This article details a method for generating genetically modified T cells using CAR and CRISPR lentiviruses. The process involves transducing T cells to express chimeric antigen receptors and editing specific genes.

Key Study Components

Area of Science

Gene editing
Immunotherapy
Cellular biology

Background

Chimeric antigen receptors (CARs) enhance T cell targeting of cancer cells.
CRISPR technology allows for precise gene editing in T cells.
Antibiotic selection is used to isolate modified cells.
Non-homologous end joining is a common DNA repair mechanism.

Purpose of Study

To develop a protocol for generating CAR T cells.
To demonstrate the use of CRISPR for gene disruption in T cells.
To provide a method for isolating genetically modified cells.

Methods Used

Transduction of T cells with CAR and CRISPR lentiviruses.
Reverse transcription of viral RNA into DNA.
Selection of modified T cells using antibiotics.
Ultracentrifugation for virus concentration.

Main Results

Successful generation of CAR T cells with targeted gene modifications.
Isolation of genetically modified cells through antibiotic selection.
Demonstration of effective gene disruption using CRISPR.
Protocol established for future CAR T cell generation.

Conclusions

The method provides a reliable approach for CAR T cell production.
CRISPR technology can be effectively utilized for gene editing in T cells.
Further applications in immunotherapy can be explored using this protocol.

Frequently Asked Questions

What are CAR T cells?

CAR T cells are genetically engineered T cells that express chimeric antigen receptors to target specific cancer cells.

How does CRISPR work in this context?

CRISPR is used to introduce specific gene edits in T cells, allowing for targeted modifications.

What is the role of antibiotics in this protocol?

Antibiotics are used to eliminate unmodified T cells, ensuring that only genetically modified cells are selected.

What is non-homologous end joining?

Non-homologous end joining is a DNA repair mechanism that can lead to insertions or deletions at the site of a double-stranded break.

What are the potential applications of this research?

This research can advance immunotherapy strategies for cancer treatment by improving the efficacy of CAR T cells.

Begin with a suspension of T cells and treat them with CAR lentiviruses carrying a gene for the chimeric antigen receptor or CAR and CRISPR lentiviruses.

The CRISPR lentivirus contains genes for the guide RNA and Cas9 nuclease as well as an antibiotic resistance gene.

Both the CAR and CRISPR lentiviruses interact with T cells and release their RNA.

These RNAs are reverse-transcribed and converted into corresponding DNA, which integrates into the T cell DNA.

This enables the synthesis of CAR proteins, guide RNAs, and Cas9 proteins.

The guide RNA forms a complex with Cas9, which specifically recognizes and binds to the target gene on the T cell DNA.

Meanwhile, Cas9 cleaves the DNA, creating a double-stranded break.

This break is repaired via non-homologous end joining, an error-prone repair mechanism, resulting in target gene modification.

This generates genetically modified T cells with chimeric antigen receptors.

Treat the cells with antibiotics to eliminate the unmodified T cells and selectively isolate the genetically modified CAR T cells.

To disrupt granulocyte-macrophage colony-stimulating factor, utilize a guide RNA, as described in the manuscript. Incubate transfection reagents at room temperature for 30 minutes. After incubation, add them to the 293T cells that have reached 70% to 90% confluency, and culture the transfected cells at 37 degrees Celsius, 5% CO₂ to produce lentivirus.

At 24 and 48 hours, harvest, and concentrate virus-containing supernatant by ultracentrifugation in 50-milliliter ultracentrifuge tubes, and freeze at minus 80 degrees Celsius for future use. Then, on day one, gently resuspend the T cells to break up rosettes.

In a BSL-2 plus approved laboratory, to generate CAR T cells, add CAR19 lentivirus and GM-CSF-targeting CRISPR lentivirus to the stimulated T cells. On day three and day five, for successfully transduced lenti-CRISPR-edited T cells carrying puromycin resistance, treat cells with puromycin dihydrochloride at a concentration of 1 microgram of puromycin per milliliter.

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