Toolkit Items

Browse the toolkit beneath workflows. The mechanism branch runs mechanism -> architecture -> component, while the technique branch runs from high-level approaches down to concrete methods.

2 items matching 1 filter

Mechanism Branch

Layer 1

Mechanisms

Top-level concepts: biophysical action modes such as heterodimerization, photocleavage, or RNA binding.

Layer 2

Architectures

Arrangements that realize or deploy mechanisms, including switches, construct patterns, and delivery strategies.

Layer 3

Components

Low-level parts and sequence-defined elements used inside architectures, including protein domains and RNA elements.

Technique Branch

Layer 1

Approaches

High-level engineering practices such as computational design, directed evolution, sequence verification, and functional assay.

Layer 2

Methods

Concrete methods used to design, build, verify, or characterize engineered systems.

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crispr/cas9 genome editing

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inducible gRNA (gRNAi) AAV vector

Construct Pattern
Since 2016crispr/cas9 genome editingdoxycycline-dependent transcriptional derepressiontetr-mediated repression of grna expressionComputational Design

The inducible gRNA (gRNAi) AAV vector is an adeno-associated viral construct that places a CRISPR guide RNA under an H1/TO promoter and co-expresses Tet repressor (TetR) for doxycycline-dependent control of gRNA expression. In the cited 2016 study, related H1/TO and U6/TO promoter configurations supported doxycycline-dependent DNA editing in vitro, and the system was described for inducible in vitro and in vivo genome editing.

CFBacMamMusHumTxRep
Ev 28Rep 9Pr 71

H1/TO promoter

Multi-Component Switch
Since 2016crispr/cas9 genome editingcrispr/cas9-mediated dna editingsmall-molecule-inducible transcriptional derepressionsmall-molecule-inducible transcriptional repression/derepressiontetracycline-operator regulationtetr-operator regulationComputational Design

The H1/TO promoter is a tetracycline-operator-modified H1 RNA polymerase III promoter used in a multi-component CRISPR/Cas9 switch to drive doxycycline-dependent guide RNA expression. In the reported system, it functioned with TetR-mediated regulation and supported in vitro DNA editing with efficiency similar to a U6/TO promoter.

CFBacMamMusHumTxRep
Ev 28Rep 9Pr 49
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