Alkaline phosphatase (AP) conjugated Anti-Bovine Primary Antibodies

Alkaline phosphatase (AP) conjugated Anti-Bovine Primary Antibodies

Alkaline phosphatase (AP)-conjugated anti-bovine primary antibodies combine highly specific recognition of bovine antigens with enzymatic signal amplification, enabling sensitive and direct detection in immunoassays. By linking antigen specificity to AP catalytic activity, these reagents eliminate the need for secondary antibodies while generating stable colorimetric, chemiluminescent, or fluorescent signals.

Enzymatic Mechanism

Alkaline phosphatase (AP, EC 3.1.3.1), commonly derived from calf intestine, catalyzes the hydrolysis of phosphate esters under alkaline conditions (optimal pH ~9.5), producing detectable signals depending on the substrate used.

  • Chromogenic substrates:
    • pNPP → yellow product (405 nm)
    • BCIP/NBT → purple precipitate (histological applications)
    • Fast Red → red precipitate (immunohistochemistry)
  • Chemiluminescent detection: Dioxetane phosphate substrates generate light emission with high sensitivity and extended signal stability.
  • Fluorescent detection: ELF-97 phosphate produces a photostable yellow-green fluorescent signal.

The enzymatic turnover of AP enables significant signal amplification, typically ranging from 100- to 1000-fold compared to direct dye conjugates, with a broad linear detection range spanning picogram to microgram levels of antigen.

Antibody Characteristics

  • Host species: Rabbit, goat, or donkey-derived immunoglobulins targeting bovine IgG (H+L), serum albumin, or specific bovine proteins.
  • Conjugation chemistry:
    • Glutaraldehyde crosslinking (formation of heterogeneous multimers)
    • DSS/BS3 crosslinkers (stable amide bond formation)
    • SMCC chemistry (thiol-maleimide coupling enabling oriented conjugation)
  • Purification strategies:
    • Affinity chromatography (Protein A/G or antigen-specific columns)
    • Cross-adsorption to minimize interspecies cross-reactivity
    • F(ab')₂ fragment generation to reduce Fc-mediated background
  • Functional properties:
    • Working titer: 1:1000 – 1:20,000 dilution range
    • Stability: up to 1 year at 4°C (with 0.1% sodium azide)
    • Molecular weight: ~160–300 kDa (due to AP multimerization)

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