BD Functional Cell-Based Reagents for Flow Cytometry & Imaging
45 productsIright brings together BD’s functional cell-based reagents and NA/LE (no-azide/low-endotoxin) antibodies so you can interrogate apoptosis, proliferation, DNA damage, and phospho-signaling with confidence. This collection page helps you pick the right dyes, kits, and phospho-targets, then jump straight into validated BD SKUs that match your workflow.
Introduction to BD Functional Cell-Based Reagents
From early cell stress to pathway activation, functional readouts reveal what surface markers alone cannot. BD’s portfolio spans apoptosis detection, cell-cycle and proliferation tools, DNA damage markers (γ-H2AX), and Phosflow™ antibodies for intracellular signaling—optimized primarily for flow cytometry and compatible with imaging, IHC, and WB where applicable. As a distributor, Iright offers genuine supply, documentation, and technical coordination.
Product Families: Apoptosis, Proliferation, DNA Damage & Phospho-Flow
Choosing among functional assays starts with the biological question. Below is a concise overview of the major families you’ll meet on this page, highlighting typical readouts and why researchers rely on BD’s formats and buffers to maintain signal quality and experimental consistency across platforms.
Apoptosis & Viability. Annexin V kits report phosphatidylserine externalization; 7-AAD or PI enables dead-cell exclusion and 2-parametric viability calls by flow cytometry. BD offers FITC or PE Annexin V kits with binding buffer for straightforward panels.
Cell-Cycle & Proliferation. For DNA content profiling and phase analysis, the BD Cycletest™ Plus kit provides nuclei staining workflows. For division tracking, pair with flow-read proliferation dyes (e.g., CFSE alternatives) or complementary gating strategies.
DNA Damage & Repair. Anti-H2AX (pS139), i.e., γ-H2AX, sensitively marks double-strand break responses and adapts to flow, imaging, or blotting with PE- or purified formats to suit your protocol.
Phospho-Signaling (Phosflow). BD Phosflow antibodies (e.g., p-STAT3 Y705) pair with dedicated lyse/fix and Perm Buffer III to quantify intracellular phosphorylation states by flow, enabling time-resolved pathway analysis in whole blood or cell lines.
Functional-grade (NA/LE) Antibodies. When you need to stimulate, block, or neutralize without sodium azide or confounding endotoxin, BD’s NA/LE format minimizes interference in sensitive in-vitro and in-vivo assays.
Selection Guide: Assay Goal, Readout, and NA/LE Antibody Choice
Before adding items to the cart, align the assay design with the output and constraints. The short guide below helps you map goals to BD reagents, buffers, and formats, and decide when NA/LE antibodies are essential to protect functional readouts from azide/endotoxin effects.
-
Define the biological question. Detect early apoptosis? Quantify dead-cell burden? Track divisions or map pathway activation after cytokine stimulation? Each goal points to distinct BD probes or phospho-targets.
-
Match the readout. Flow cytometry remains primary for Annexin V/7-AAD, Cycletest DNA content and Phosflow; γ-H2AX can extend to imaging and WB for orthogonal confirmation.
-
Decide on fixation/permeabilization. Apoptosis/viability is generally live-cell (no fixation before staining), whereas Phosflow requires lyse/fix and BD Perm Buffer III; plan panel order accordingly.
-
Use NA/LE when function matters. For blocking/activation or co-culture systems, choose NA/LE antibodies to avoid azide toxicity and endotoxin artifacts that skew proliferation or cytokine-response data.
- Build controls and time points. Include untreated, positive inducers (e.g., camptothecin for apoptosis; IL-6 for p-STAT3), FMO/compensation controls, and staged time courses to capture dynamics with confidence.
Comparison Table: Dyes, Kits, Phospho Antibodies & NA/LE Formats
The matrix below summarizes common choices. Use it to shortlist items before drilling into specifications and IFUs. Consider sample type, compatibility with fixation, and whether RUO reagents meet your compliance needs.
| Subfamily / Use | Core Target / Probe | Primary Readout | Fix/Perm Needed | NA/LE Option | Typical Sample | Representative BD Item |
|---|---|---|---|---|---|---|
| Early apoptosis + viability | Annexin V + 7-AAD | Flow | No (live stain) | N/A | Cell lines, PBMCs | FITC Annexin V Apoptosis Detection Kit I (556547); PE Annexin V Kit I (559763) |
| Dead-cell exclusion | 7-AAD | Flow | No (endpoint stain) | N/A | Broad | 7-AAD (559925) |
| DNA content / cell-cycle | Propidium iodide-based kit | Flow | Yes (nuclear prep) | N/A | Tissue, suspensions | Cycletest™ Plus DNA Reagent Kit (340242) |
| DNA damage (DSB response) | H2AX (pS139) / γ-H2AX | Flow / Imaging / WB | Depends on assay | N/A | Broad | Purified anti-H2AX (pS139) (560443); PE anti-H2AX (pS139) (562377) |
| Phospho-signaling | STAT3 (pY705) | Flow (Phosflow) | Yes (Lyse/Fix + Perm III) | N/A | Whole blood, cells | BD Phosflow PE anti-STAT3 (pY705) (612569); Perm Buffer III (558050) |
| Functional modulation | NA/LE functional-grade mAbs | Functional assays | No | Yes | In-vitro / in-vivo | NA/LE Mouse anti-human CD11b (555385); NA/LE panel list (see BD NA/LE PDF) |
Protocol Tips & FAQs: Panel Design, Controls, Compensation
As functional assays touch viability, fixation, and intracellular targets, careful order-of-operations and controls are essential. The notes below condense BD-documented practices so you can spend time on biology—not troubleshooting artifacts.
1. How should I order live-cell and fixed-cell steps?
Perform Annexin V/7-AAD on live cells prior to any fixation. For phospho-targets, follow BD Phosflow workflow: stimulation → Lyse/Fix → Perm Buffer III → intracellular stain. Keep apoptosis and phospho-assays separate or use compatible panels with strict timing.
2. What positive controls are recommended?
Classic inducers include camptothecin for apoptosis (Annexin V kits provide an example with Jurkat cells) and IL-6 for STAT3 phosphorylation. Build time courses (e.g., 5–30 minutes for phospho-events; 3–6 hours for apoptosis) to capture kinetics.
3. When is NA/LE mandatory?
Any experiment where azide or endotoxin can blunt or confound function—e.g., T-cell activation, blocking/neutralization, co-culture, or in-vivo dosing—should use NA/LE antibodies to avoid toxicity or innate activation from contaminants.
4. How do I prevent spectral spillover and low signal-to-noise?
Use FMO and single-stained controls; avoid fluorophore crowding in adjacent channels; titrate antibodies; minimize light exposure for dyes; and for methanol-perm steps (Perm III), mind epitope sensitivity and wash thoroughly.
5. What about WB/imaging confirmation?
γ-H2AX can be validated by WB (~15 kDa band) or imaged in nuclei as an orthogonal check on flow findings; ensure fixation/permeabilization is compatible with your chosen format (purified vs PE-conjugate).
Talk to Iright
If you’re planning a multiparameter panel or moving from discovery to verification, we can help you finalize clones, fluor mixes, and buffer kits—and provide quotes with delivery windows. Tell us your instrument, sample type, and target pathways; we’ll confirm BD catalog numbers, RUO status, and provide data-sheet bundles for your records.
What you get from Iright
- Genuine BD supply with matched catalog numbers and IFU/technical data sheets.
- Assistance aligning Lyse/Fix & Perm III workflows with your panel and viability strategy.
- Guidance on NA/LE choices for blocking/activation and in-vivo compatibility.
Order Guidelines
1. Price & Stock Available on Request. Click to send email to: service@iright.com
2. Please DO NOT make any payment before confirmation.
3. Minimum order value of $1,000 USD required.
4. 100% prepayment required.
Collaboration
Tony Tang
Email: Tony.Tang@iright.com
Mobile/WhatsApp/Wechat: +86-17717886924
