scAAV-Synapsin-GFP (AAV Serotype DJ, Self-complementary)

What it means: Promoter is the DNA regulatory element that drives transcription of the AAV payload. The promoter listed here is Synapsin.

How to interpret here: Use Synapsin to predict where and how strongly your transgene will be expressed. Promoters vary in strength, cell-type preference, and long-term stability in different tissues. Expression regulation is listed as Constitutive—this affects whether expression is always on vs controlled by a system/design. Cell-type intent is Neurons—promoter choice is one of the main drivers of specificity, but serotype and delivery route also shape which cells are transduced. Serotype is AAV2/DJ—capsid tropism can limit which cells ever receive the genome, even with a broadly active promoter. Transgene is GFP—very high expression of some payloads can be toxic or confounding, so promoter strength should match your biology. Listed applications: In vivo gene delivery, Cell labeling, Promoter testing, Transduction benchmarking. If your goal is in vivo work, consider promoter suitability for your tissue and timeline.

Why it matters for buying:

• Specificity: Promoter choice is the main lever for restricting expression to certain cell types (when possible).
• Signal level: Promoter strength influences detectability, functional effect size, and risk of overexpression artifacts.
• Design constraints: Promoter size competes with payload size inside AAV packaging limits, which can force trade-offs.

Practical guidance:

• Match promoter to tissue: Choose promoters with known performance in your tissue/model (especially for in vivo brain work).
• Plan validation: Confirm expression pattern with a reporter or immunostaining early (pilot cohort) before committing to a large study.
• Consider immune/silencing effects: Some promoters can behave differently over time in vivo—monitor expression at the timepoints you care about.

What to watch out for:

• Promoter ≠ tropism: A promoter can’t drive expression in cells that aren’t transduced; serotype/route still control delivery.
• Context dependence: Promoter activity can change with developmental stage, disease state, or inflammation.
• Overexpression: Very strong promoters can produce non-physiologic levels—interpret phenotypes with dose and controls.

Handling note:

• Form: Frozen liquid — plan thawing/mixing accordingly and avoid repeated freeze-thaw where possible.
• Buffer: Sterile PBS — confirm compatibility with your injection/assay buffer requirements.
• Storage: -80°C — aliquot on first thaw when feasible to preserve titer/activity.

What it means: Transgene is the gene payload carried by the AAV genome (the coding sequence or functional cassette). The transgene listed here is GFP.

How to interpret here: Use GFP to determine what biological function you’re introducing (overexpression, recombinase, reporter, sensor, or control). The same serotype/promoter can behave very differently depending on payload biology. GFP/eGFP payloads are commonly used for transduction mapping, expression verification, and cell labeling. Function category is Control/Fluorescent Proteins—use this to sanity-check that the payload matches your experimental intent. Promoter is Synapsin—promoter strength and specificity control where the transgene is expressed. Expression regulation is Constitutive—verify whether your design expects constitutive vs regulated expression. Reporter/tag is GFP—this affects how you verify expression (imaging, flow, immunostaining). Cellular localization is Cytosolic—confirm it matches your assay readout (nuclear vs cytosolic vs membrane).

Why it matters for buying:

• Biological relevance: The transgene defines the mechanism you’re testing—incorrect payload choice can invalidate the study design.
• Assay compatibility: Some payloads require specific detection, stimulation, or genetic context (e.g., Cre/lox).
• Safety and artifacts: High expression or active enzymes can stress cells; dose and controls matter.

Practical guidance:

• Confirm compatibility: For recombinases/editors, verify your model (floxed allele/reporter) and any required guide RNA or helper systems.
• Plan a pilot: Validate expression and basic function (timecourse, dose range) before committing to large cohorts.
• Use matched controls: Include a null/control vector and/or a reporter-only control to separate delivery effects from payload effects.

What to watch out for:

• Payload-dependent toxicity: Some genes/sensors are sensitive to expression level—avoid assuming “more is better.”
• Interpretation drift: Reporters show expression, not necessarily functional effect—pair with functional readouts.
• Genetic context: Cre/Flp effects depend on the target locus and recombination efficiency.

Handling note:

• Form: Frozen liquid — plan thawing/mixing accordingly and avoid repeated freeze-thaw where possible.
• Buffer: Sterile PBS — confirm compatibility with your injection/assay buffer requirements.
• Storage: -80°C — aliquot on first thaw when feasible to preserve titer/activity.

What it means: Reporter/Tag describes a reporter protein and/or an epitope tag included for detection, tracking, or localization. The value shown here is GFP.

How to interpret here: Use GFP to decide how you will verify expression (fluorescence imaging, immunostaining, flow cytometry, Western blot, etc.) and whether the tag might influence the biology of the payload. GFP-family reporters enable direct fluorescence imaging; protect samples from photobleaching and match filter sets to the reporter. Transgene is GFP—confirm whether the reporter/tag is separate (co-expression) or fused, since fusions can change localization or function. Cellular localization is Cytosolic—a reporter/tag can be your readout for correct compartment targeting. Listed applications: In vivo gene delivery, Cell labeling, Promoter testing, Transduction benchmarking—choose detection methods compatible with your workflow and sample type.

Why it matters for buying:

• Verification: Reporters/tags reduce ambiguity by showing where and how strongly the vector is expressed.
• Workflow: Your equipment (microscope/flow/imager) must match the reporter’s spectral properties or antibody reagents.
• Biology: Tags and fusions can alter localization or activity; interpretation needs controls.

Practical guidance:

• Match detection to reporter: Confirm excitation/emission filters for fluorescent proteins or validated antibodies for epitope tags.
• Include controls: Use vector-only and detection-only controls (e.g., no-primary controls for IHC/IF) to manage background.
• Check fusion effects: If your assay depends on native function, consider whether a fusion tag could interfere and validate functionality.

What to watch out for:

• Autofluorescence: Some tissues have high background; choose reporters accordingly and validate signal-to-noise.
• Spectral overlap: Multiplex imaging/flow requires compensation and careful channel planning.
• Tag accessibility: Tags may be masked by folding or fixation—validate detection conditions.

Handling note:

• Form: Frozen liquid — plan thawing/mixing accordingly and avoid repeated freeze-thaw where possible.
• Buffer: Sterile PBS — confirm compatibility with your injection/assay buffer requirements.
• Storage: -80°C — aliquot on first thaw when feasible to preserve titer/activity.

What it means: Function summarizes the intended experimental role of this AAV design (e.g., control, labeling, perturbation). The value shown here is Control/Fluorescent Proteins.

How to interpret here: Use Control/Fluorescent Proteins to decide whether this is an appropriate experimental control or an active biology-changing reagent. Function categories are often broader than the specific payload, so cross-check with the transgene and promoter. Control vectors are used to match delivery, promoter activity, and capsid exposure without confounding biological activity from an experimental payload. Transgene is GFP—this is the most concrete indicator of mechanism (e.g., reporter vs recombinase vs effector). Reporter/tag GFP can help verify expression, which is especially useful for controls and benchmarking. Listed applications: In vivo gene delivery, Cell labeling, Promoter testing, Transduction benchmarking—align the function with your workflow (in vivo delivery vs in vitro benchmarking).

Why it matters for buying:

• Study design: Function determines whether the vector is a control, a readout tool, or an intervention.
• Interpretability: Using the right control reduces ambiguity (delivery/capsid effects vs payload effects).
• Cost efficiency: Selecting an appropriate control vector can save time by preventing confounded experiments.

Practical guidance:

• Choose controls that match: For in vivo work, match serotype and promoter when using a control vector so delivery and expression context are comparable.
• Define your readout: Decide whether you need a reporter to verify expression distribution and kinetics.
• Document dosing: Record vg dose, route, and timepoint so results are comparable and reproducible.

What to watch out for:

• Control mismatch: A control with a different promoter/serotype can mislead by changing transduction patterns.
• Reporter effects: Even ‘neutral’ reporters can affect cell physiology at very high expression; interpret carefully.
• Context dependence: Function categories don’t guarantee outcomes—validate in your model.

Handling note:

• Form: Frozen liquid — plan thawing/mixing accordingly and avoid repeated freeze-thaw where possible.
• Buffer: Sterile PBS — confirm compatibility with your injection/assay buffer requirements.
• Storage: -80°C — aliquot on first thaw when feasible to preserve titer/activity.

What it means: Cell Type indicates the intended or typical cell population for expression/readout. The value shown here is Neurons.

How to interpret here: Use Neurons as a guide for expected expression patterns, but treat cell-type targeting as a combination of promoter choice, capsid/serotype tropism, route, and dose—not a single-field guarantee. Neuron-biased designs often pair neuronal promoters with neurotropic serotypes; validate specificity with marker co-staining if cell-type restriction is critical. Promoter is Synapsin—promoter is the primary driver of cell-type restriction when applicable. Serotype is AAV2/DJ—serotype affects which cells are transduced; a cell-type promoter won’t help if the capsid doesn’t reach/enter the target cells. Expression regulation is Constitutive—regulation can affect when and where expression is observed. Listed applications: In vivo gene delivery, Cell labeling, Promoter testing, Transduction benchmarking—plan validation (marker co-staining, reporter imaging) in the relevant tissue and timepoint.

Why it matters for buying:

• Specificity: Correct cell-type targeting reduces off-target expression and improves interpretability.
• Efficiency: Cell populations vary in transduction efficiency; design and route choices affect required dose and success rate.
• Controls: Cell-type assumptions drive what controls and validation markers you need.

Practical guidance:

• Validate cell identity: Use marker co-localization (immunostaining or genetic reporters) to confirm which cells express the payload.
• Optimize delivery: Route, dose, and timing can shift cell-type distribution—pilot studies are highly recommended.
• Plan background controls: Include vector-only/null controls and assess off-target expression in non-target cell populations.

What to watch out for:

• Species and age effects: Tropism and promoter behavior can vary across species, strain, and developmental stage.
• Inflammation/disease: Disease states can change promoter activity and cell susceptibility to transduction.
• Over-interpretation: ‘Cell type’ labels are guidance; confirm empirically in your own model.

Handling note:

• Form: Frozen liquid — plan thawing/mixing accordingly and avoid repeated freeze-thaw where possible.
• Buffer: Sterile PBS — confirm compatibility with your injection/assay buffer requirements.
• Storage: -80°C — aliquot on first thaw when feasible to preserve titer/activity.