설명
This kit contains recombinant Mouse M-CSF and Mouse RANKL, designed to induce the differentiation of mouse-derived precursor cells (such as the RAW264.7 cell line or primary bone marrow mononuclear cells) into mature osteoclasts with functional bone-resorbing capability.
M-CSF (Macrophage Colony-Stimulating Factor) supports the survival and proliferation of precursor cells and primes them for osteoclast differentiation, serving as the "licensing" signal. RANKL (Receptor Activator of Nuclear Factor Kappa-B Ligand) is the decisive signal driving the terminal differentiation and fusion of osteoclasts, activating key downstream transcription programs such as NFATc1.
The M-CSF and RANKL included in this kit are characterized by high activity, high purity, and low endotoxin levels. This kit efficiently drives the differentiation of precursor cells into osteoclasts, yielding a large number of mature, multinucleated, TRAP-strong positive osteoclasts.
Product Information
|
Product Information. |
Catalog Number |
Size |
|
Mouse Osteoclast Cell Differentiation Cytokine Set |
92649ES10 |
10 μg |
|
92649ES50 |
50 μg |
Components
|
Component Cat No. |
Component Name |
92649ES10 |
92649ES50 |
|
92649ES-A |
Mouse M-CSF Protein |
10 μg |
50 μg |
|
92649ES-B |
Mouse RANKL Protein |
25 μg |
100 μg |
Product Includes
|
Component Cat No. |
Product Name |
Recommended Concentration |
Source |
Appearance |
Quantity |
|
91114ES |
Mouse M-CSF Protein |
50 ng/mL |
E.coli |
Lyophilized Powder |
1 |
|
95625ES |
Mouse RANKL Protein |
100 ng/mL |
HEK293 |
Lyophilized Powder |
1 |
Reconstitution Method
|
Component Name |
Reconstitution Method |
|
Mouse M-CSF Protein |
Prior to opening the vial, centrifuge to ensure the contents are collected at the bottom. Reconstitute with sterile distilled water or PBS to a concentration of 0.1–1.0 mg/mL. The solution may be further diluted according to subsequent experimental requirements. For long-term storage, it is recommended to add a carrier protein (0.1% BSA) to the dilution buffer. Aliquot into single-use volumes and store at -80°C. Avoid repeated freeze-thaw cycles. |
|
Mouse RANKL Protein |
Centrifuge before opening. Reconstitute the lyophilized protein with distilled water to a concentration greater than 100 μg/mL. It is recommended to aliquot the protein into single-use portions upon first use to avoid repeated freeze-thaw cycles. |
Storage
Long-term Storage: Store at -25 ~ -15°C. Valid for 1 year from the date of receipt.
Reconstituted (Short-term): After reconstitution, store under sterile conditions at 2 ~ 8°C for up to 7 days.
Reconstituted (Long-term): After reconstitution, store under sterile conditions at -85 ~ -65°C for up to 3 months.
Product Properties
|
Source Species |
Mouse |
|
Tag |
No Tag |
|
Expression System |
HEK293 |
|
Endotoxin |
< 1.0 EU per μg by the LAL method. |
|
Formulation |
Lyophilized from 0.22 μm filtered solution in PBS (pH 7.4). |
|
Appearance |
Lyophilized Powder |
Notes
1. For your safety and health, please wear a lab coat and disposable gloves during operation.
2. This product is for research use only.
Protocol
Protocol for Osteoclast Differentiation from RAW 264.7 Cells
1. Seeding of Osteoclast Precursors
1.1 Cell Preparation: Harvest RAW 264.7 cells in good growth condition and resuspend them in complete
α -MEM medium supplemented with 10% Fetal Bovine Serum (FBS). Perform cell counting.
1.2 Seeding: Seed the cells into a 24-well culture plate containing sterile glass coverslips at a density of
2.5×103 cells/mL. Add 1 mL of cell suspension to each well.
1.3 Adherence: Incubate the plate in a humidified incubator at 37°C with 5% CO₂ for 18 hours to allow cell attachment.
2. Osteoclast Induction and Differentiation
2.1 Medium Replacement: Approximately 18 hours after seeding, once the cells have attached, carefully aspirate the old medium from the wells.
2.2 Induction: Replace with fresh complete osteoclast induction medium. This medium consists of α -MEM supplemented with 10% FBS, 50 ng/mL recombinant Mouse M-CSF Protein, and 100 ng/mL recombinant Mouse 2.3 RANKL Protein. Maintenance: Change the induction medium every 3 days. During each change, gently aspirate the spent medium and replace it with an equal volume of fresh induction medium containing the same concentrations of M-CSF and RANKL.
3. Morphological Observation and Identification
3.1 Morphology: Observe morphological changes regularly under an inverted microscope starting from the beginning of induction. Typically, typical multinucleated osteoclast-like structures can be observed after 4 days of RANKL induction.
3.2 TRAP Staining: After 5 days of RANKL induction, perform Tartrate-Resistant Acid Phosphatase (TRAP) staining to specifically identify osteoclasts. Strictly follow the manufacturer's instructions for the TRAP staining kit.
Result Interpretation: Observe under a light microscope after staining. Mature osteoclasts will exhibit a red or reddish-purple cytoplasm.
Documents:
Manuals:
결제 및 보안
귀하의 결제 정보는 안전하게 처리됩니다. 당사는 신용카드 정보를 저장하지 않으며 귀하의 신용카드 정보에 접근할 수 없습니다.
당신은 또한 좋아할 수 있습니다
문의
자주 묻는 질문
이 제품은 연구 목적으로만 사용되며 인간이나 동물의 치료 또는 진단용으로 의도되지 않았습니다. 제품과 콘텐츠는
특정 애플리케이션에는 추가적인 제3자 지적 재산권이 필요할 수 있습니다.
예슨은 윤리적 과학에 헌신하며, 우리의 연구가 안전과 윤리적 기준을 보장하는 동시에 중요한 문제를 해결해야 한다고 믿습니다.

