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CRISPR 101: Any Base Transversion Editors

By Emily P. Bentley

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CRISPR 101

CRISPR 101: Cytosine Transversion Editors

Emily P. Bentley March 25, 2025

The first base editors revolutionized CRISPR gene editing. Cytosine base editors (CBEs) and adenine base editors (ABEs) chemically modify target bases without breaking the DNA backbone, making them efficient and precise tools for altering DNA sequences. These first base editors ...
The nucleobases are shown with arrows describing conversions between them. In step one, a cytosine deaminase converts cytosine to uracil; this is catalyzed directly by the base editor. Next, base excision of uracil (also by the base editor) is repaired in two different ways by the cell, shown by an arrow that splits into two outcomes. Repair in E. coli leads to adenine, while repair in mammalian cells leads to guanine.
CRISPR

Typing CRISPR Systems

Alyssa Shepard March 18, 2025

What’s in a type? That which we call CRISPR, by any other name would…probably still edit genomes.
A schematic overview of the CRISPR classification system.
Hot Plasmids

Hot Plasmids: Winter 2025

Multiple Authors March 11, 2025

Every few months, we highlight some of the new plasmids, antibodies, and viral preps in the repository through our Hot Plasmids articles.

Reflections and Looking Ahead

Chonnettia Jones February 25, 2025

Twenty years of accelerating scientific discovery. Over 150,000 plasmids empowering researchers worldwide. Countless breakthroughs enabled by shared resources. As we step into 2025, these milestones remind us of the extraordinary impact that happens when scientists come together ...
CRISPR

CRISPR 101: Cytosine and Adenine Base Editors

Multiple Authors February 13, 2025

Early CRISPR applications were often limited by the low editing efficiency of homology-directed repair (HDR), the pathway for resolving DNA double-strand breaks (DSBs) preferred by researchers. Compared to non-homologous end joining (NHEJ), HDR occurs at a relatively low ...
A cartoon depiction of cytidine base editing. A base editor, consisting of a cytidine deaminase fused to Cas9, is shown binding to DNA using its guide RNA. The guide RNA base pairs to target DNA, leaving the opposite strand of DNA free to be contacted by the cytidine deaminase, which converts a C to a U within this single-stranded sequence. This deamination yields DNA with a G:U mismatch without creating a double-strand break. Mismatch repair preserves the edit IF the modified strand is used as the template, converting the mismatched G to an A and yielding a single-base-pair edit.
CRISPR

Degrading DNA with Cascade-Cas3

Alyssa Shepard February 11, 2025

The versatility of CRISPR allows you to play with DNA in a number of ways, from small edits that change single base pairs, to chromosomal inversions and large deletions. Many of these methods rely on Cas9 or a derivative of Cas9, but the ever-expanding repertoire of CRISPR has ...
Diagram of the Cascade complex with gRNA bound to target DNA, after recruitment of Cas3. Cas3 is about to nick the non-target strand.
Addgene News

Export Control Regulations Lifted for Plasmids Containing Rabies and VSV-G Genes

Rachel Leeson February 6, 2025

If you're an international researcher who uses plasmids containing genes from rabies and vesicular stomatitis virus, you may have noticed it’s been easier to order these plasmids. This is because in 2024 certain export control exceptions were made by the US Bureau of Industry ...

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