Porcine Primary Coronary Artery Smooth Muscle Cells

SKU:BHC10923241
Suppliers
Applied Biological Materials (abm) Inc.
Applied Biological Materials (abm) Inc.
Details Products
Overview
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Porcine Primary Coronary Artery Smooth Muscle Cells are porcine frozen primary cells from blood vessel for vascular remodeling, contractile signaling, and smooth muscle phenotypic regulation studies. Key attributes include adherent, polygonal; recommended seeding density is 15,000 cells/cm².
Species Pig
Cell Type Primary Cells
Tissue Blood Vessel
Growth Adherent, polygonal
Format Frozen
Options selector
Catalog no. Pack Size
T5000 5x105 cells / 1.0 ml
Available Options

Select the variant that best fits your experiment. Availability and lead time may vary by option.

  • Options: Pack Size: 5x105 cells / 1.0 ml
  • Lead time: varies by selected option; please contact us for current fulfillment timing.
  • Storage: Vapor phase of liquid nitrogen, or below -130°C. Cryopreservation: We recommend using serum-free CryoGuard™ Freezing Media (TM078). Upon receipt: Transfer to liquid nitrogen vapor phase or below -130°C until use; thaw and initiate culture as soon as possible upon receipt; do not store at -70°C.
  • Shipping: Ship with dry ice.
  • Upon receipt: store at the recommended temperature as soon as possible.
  • Sales terms and conditions: Please review prior to ordering.
Field Specification
Mfr No T5000
Product Format Frozen
Product Type
  • Cells
  • Primary Cells
Shipping Ship with dry ice.
Storage Vapor phase of liquid nitrogen, or below -130°C. Cryopreservation: We recommend using serum-free CryoGuard™ Freezing Media (TM078). Upon receipt: Transfer to liquid nitrogen vapor phase or below -130°C until use; thaw and initiate culture as soon as possible upon receipt; do not store at -70°C.

Overview

Porcine Primary Coronary Artery Smooth Muscle Cells are porcine frozen primary cells from blood vessel used for vascular remodeling, contractile signaling, and smooth muscle phenotypic regulation studies. These cells display adherent, polygonal growth characteristics.

Key elements and design rationale

  • Biological source: Pig (Porcine)
  • Tissue origin: Blood Vessel
  • Growth properties: Adherent, polygonal
  • Format: Frozen
  • Seeding guidance: 15,000 cells/cm²
  • Biosafety level: II
  • Culture context: For optimal cell culture, we recommend using PriCoat™ T25 Flasks (G299) or coating your preferred vessels with Applied Cell Extracellular Matrix (G422) . PriGrow X Series Medium (TM5000) + 1% Penicillin/Streptomycin Solution (G255), 37.0°C, 5% CO₂

Smooth muscle cells regulate vessel tone, extracellular matrix remodeling, and responses to growth factors, cytokines, and mechanical cues. In culture, they are often used to study contractile-to-synthetic state transitions.

Research relevance and current trends

  • Studies frequently examine how inflammatory, mechanical, or metabolic cues alter smooth muscle phenotype and matrix production.
  • Primary vascular smooth muscle cells are used to model remodeling pathways relevant to stenosis, calcification, and vascular injury.
  • Comparative donor and vessel-source studies help capture regional heterogeneity across the arterial tree.

Common research applications

  • Measure contractile marker expression or phenotype switching after defined perturbations.
  • Evaluate proliferation, migration, and matrix-remodeling responses in vascular remodeling models.
  • Use in co-culture with endothelial cells or fibroblasts to examine vessel wall signaling.

Product-specific data supplied for this listing

  • Growth Conditions: For optimal cell culture, we recommend using PriCoat™ T25 Flasks (G299) or coating your preferred vessels with Applied Cell Extracellular Matrix (G422) . PriGrow X Series Medium (TM5000) + 1% Penicillin/Streptomycin Solution (G255), 37.0°C, 5% CO₂
  • Warranty: abm warrants that cell lines shall be viable upon initiation of culture for a period of thirty (30) days after shipment and that they shall meet the specifications on the applicable abm Material Product Information sheet, certificate of analysis, and/or catalog description. Such thirty (30) day period is referred to herein as the "Warranty Period”.
  • Disclaimer: 1. Sale of this item is subjected to the completion of a Material Transfer Agreement (MTA) by the purchasing individual/institution for each order. If you have any questions regarding this, please contact us at orders@biohippo.com.
  • Seeding Density (cells/cm²): 15,000

Notes for experimental interpretation

  • Primary cells can show donor-dependent and passage-dependent variation, so morphology, growth rate, and marker expression should be interpreted in the context of the specific lot and culture history.
  • Attachment matrix, medium formulation, and gas conditions can materially influence phenotype maintenance and experimental readouts; use the recommended culture system where possible.
  • Cryopreserved recovery conditions matter for viability and downstream behavior. We recommend using serum-free CryoGuard™ Freezing Media (TM078).

SKU:BHC10923241

🧊 Thawing Protocol
  1. Thaw cells quickly in a 37°C water bath while agitating gently (maximum 2 minutes). The vial cap should be kept above the water level to minimize the risk of contamination.
  2. Decontaminate the vial by spraying and wiping the exterior of the vial with 70% ethanol. From this point onwards, all operations should be strictly carried out inside a biological safety cabinet using aseptic conditions.
  3. Transfer the cell suspension into T75 flask with 15 ml of pre-warmed complete media. Rock the flask gently to evenly distribute the cells.
  4. Incubate the cells at the recommended conditions. Do not disturb for 24 hours.
  5. Change media every 2 days until cells reach 60% confluency. Double the growth media volume when cells reach >60% confluency.
🔬 Subculture Protocol
Volumes given below are for a T75 flask; proportionally increase or decrease the volume as required per culture vessel size. Subculture cells once the culture vessel is 80% confluent.
  1. Aspirate the culture media, and add 2-3ml of pre-warmed 0.25% Trypsin-EDTA to the culture vessel.
  2. Observe the cells under a microscope to confirm detachment (typically within 2-10 minutes). Cells that are difficult to detach can be put in 37°C, for several minutes to facilitate detachment.
  3. Neutralize Trypsin-EDTA by adding an equal volume of Trypsin Neutralizing Solution (TM069) into the culture vessel.
  4. Transfer the culture suspension into a sterile centrifuge tube, and centrifuge at 125xg for 5 minutes. The actual centrifuge duration and speed may vary depending on the cell type.
  5. Aspirate the supernatant, and re-suspend the pellet with pre-warmed fresh complete growth media. Add appropriate aliquots of the cell suspension to new culture vessels, as desired.
  6. Incubate the cells at the recommended conditions.

Cell line sourcing and selection (species, tissue, and disease model matching) · Stable cell line engineering (overexpression, knockdown, knockout via CRISPR/Cas9, shRNA, sgRNA) · Reporter gene integration (GFP, RFP, luciferase, fluorescent/bioluminescent constructs) · Genome editing and knockin (point mutations, tagged endogenous proteins, conditional alleles) · Inducible expression systems (Tet-On/Off and regulatable constructs) · Drug resistance marker selection (puromycin, G418, hygromycin, and others) · Custom growth and media optimisation for specific assay requirements · Scale-up production for high-throughput screening campaigns · Authentication and QC services (STR profiling, mycoplasma testing, viability assessment). Talk to a Scientist or contact support@biohippo.com.

Do I need Applied Cell Extracellular Matrix (G422) if I am using PriCoat™ flasks?
Please refer to the Growth Conditions section of your specific product page. This section will indicate whether Applied Cell Extracellular Matrix (G422), PriCoat™ flasks, or both are recommended for optimal cell attachment and growth, as requirements may vary by cell type.
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