Human procollagen Ⅰ N-terminal peptide,PⅠNP ELISA Kit

SKU:BHE10503872
Overview
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Quantitative ELISA kit for measuring human procollagen Ⅰ N-terminal peptide (PⅠNP) in serum, plasma, and tissue homogenates to support others studies. Sensitivity 4.68 pg/mL, detection range 18.75 pg/mL–1200 pg/mL, typical assay time 1–5 h.
Target Procollagen Ⅰ N Terminal
Species Homo sapiens (Human)
Sample Type(s) serum, plasma, tissue homogenates
Assay Type Sandwich ELISA (quantitative)
Sensitivity 4.68 pg/mL
Detection Range 18.75 pg/mL-1200 pg/mL
Assay Time 1-5h
Options selector
Catalog no. Size
CSB-E11226h-96T 96 T
CSB-E11226h-96TX5 96 T×5
CSB-E11226h-96TX10 96 T×10
Available Options

Select from the available variant options shown for this product. Availability and lead time can vary by option.

  • Options: Size (96 T, 96 T×10, 96 T×5).
  • Lead time: options listed as "In Stock at Manufacturer" typically ship in 5–7 business days; other statuses may take longer.
  • Storage: refer to the product datasheet for storage and handling.
  • Sales terms and conditions: Please review prior to ordering.
Field Specification
Mfr No CSB-E11226h
Alternative Names procollagen 1 N-terminal peptide,P1NP, procollagen I N-terminal peptide,PINP
Assay Time
  • 1-5h
Assay Type
  • Sandwich ELISA (quantitative)
Detection Range 18.75 pg/mL-1200 pg/mL
Detection Wavelength 450 nm
Product Type
  • ELISA Kits
Reactivity
  • Human
Sample Type(s) serum, plasma, tissue homogenates
Sensitivity 4.68 pg/mL
Species Homo sapiens (Human)
Target Procollagen Ⅰ N Terminal

Background

procollagen Ⅰ N-terminal peptide (PⅠNP) is a biological molecule commonly studied in others research. It is commonly used as a molecular readout in mechanistic and biomarker-focused studies.

Biological context

Researchers often monitor procollagen Ⅰ N-terminal peptide in serum, plasma, and tissue homogenates to better understand themes such as mechanistic biology studies, biomarker-focused profiling, and disease-model research. In many model systems, measured levels can shift with physiology, experimental perturbation, or disease-associated changes, making careful biological interpretation important.

Interpreting changes in measured levels

Depending on sample matrix and study design, increases or decreases in procollagen Ⅰ N-terminal peptide may reflect differences in expression, secretion, turnover, or compartmentalization rather than a single mechanism. Interpretation is typically strengthened by evaluating related molecules (for example, complementary pathway markers and controls appropriate to the biological model) and by keeping pre-analytical variables consistent across groups.

Nomenclature

In publications and databases, procollagen Ⅰ N-terminal peptide may also appear under names such as procollagen 1 N-terminal peptide,P1NP, and procollagen I N-terminal peptide,PINP. When comparing studies, confirm that the reported analyte refers to the same molecule and species context.

Why ELISA data are widely used

ELISA is a common approach for quantitative measurement of proteins and biomarkers in complex samples, enabling comparisons across experimental groups and time points. When integrating results with other readouts, consider species biology, sample type, and the broader pathway context that procollagen Ⅰ N-terminal peptide participates in.

Can’t Find What You’re Looking For? We can help you source the best match or customize an ELISA solution for your study. Options may include alternative target synonyms, different species reactivity, sample type/matrix compatibility (serum/plasma/lysate/supernatant), assay format (sandwich/competitive), sensitivity/range, detection chemistry (colorimetric/fluorescent/chemiluminescent), plate format (pre-coated/uncoated, strips vs full plate), and bulk or custom packaging. Click Talk to a Scientist to submit a request form, email us at support@biohippo.com, or explore our Research Services for additional support. Our team will be in contact with you shortly.

Bone metabolism and inflammatory biomarkers in radiographic and non-radiographic axial spondyloarthritis patients: a comprehensive evaluation

I Gómez-García,Frontiers in endocrinology,2024

Changes in bone turnover markers in patients without bone metastases receiving immune checkpoint inhibitors: An exploratory analysis

F Pantano,Journal of bone oncology,2022

Praeruptorin B inhibits osteoclastogenesis by targeting GSTP1 and impacting on the S-glutathionylation of IKKβ

K Xu,Biomedicine & pharmacotherapy,2022

Three-Dimensional Co-Culture System of Human Osteoblasts and Osteoclast Precursors from Osteoporotic Patients as an Innovative Model to Study the Role of Nutrients: Focus on Vitamin K2

Domitilla Mandatori,Nutrients,2021

Increasing Vegetable Intake Decreases Urinary Acidity and Bone Resorption Marker in Overweight and Obese Adults: An 8-Week Randomized Controlled Trial

JJ Cao,The Journal of nutrition,2021

TAZ inhibits osteoclastogenesis by attenuating TAK1/NF-κB signaling

W Yang,Bone Research,2021

Citrate Supplementation Restores the Impaired Mineralisation Resulting from the Acidic Microenvironment: An In Vitro Study

N Swilam,Nutrients,2020

Umbilical cord N-terminal procollagen of type l collagen (P1NP) and beta C-terminal telopeptide (βCTX) levels in term pregnancies with vitamin D deficiency

M Eraslan Sahin,Journal Gynecological Endocrinology,2020

Association between bile acid metabolism and bone mineral density in postmenopausal women

Zhao YX,Clinics (Sao Paulo),2020

Dissecting the mechanisms of bone loss in Gorham-Stout disease

Michela Rossi, et al,Bone,2019

Spine bone mineral density increases after 6 months of exclusive lactation, even in women who keep breastfeeding

Cooke-Hubley S.et al,Arch Osteoporos,2017

Physical activity and hypocaloric diet recovers osteoblasts homeostasis in women affected by abdominal obesity

Viviana M.et al,Springer US,2016

Effect of chronic activity-based therapy on bone mineral density and bone turnover in persons with spinal cord injury

Astorino TA et al,Eur J Appl Physiol,2013

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