Osteoclast Culture Kit

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Osteoclast Culture Kit

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K-ASSAY KAMIYA BIOMEDICAL COMPANY Osteoclast Culture Kit For the culture of Osteoclasts from precursor cells. Cat. No.: CC-107 Rat Osteoclast Precursor Cells, V-1 CC-109 Mouse Osteoclast Precursor Cells, V-1 For Research Use Only. 1 Rev. 100307

K-ASSAY KAMIYA BIOMEDICAL COMPANY PRODUCT INFORMATION Cat. No. Osteoclast Culture Kit / Bone Resorption Assay CC-007 Rat Osteoclast Precursor Cells, V-1 CC-009 Mouse Osteoclast Precursor Cells, V-1 PRINCIPLE The morphogenesis and remodeling of bone requires the synthesis of bone matrix by osteoblasts and its coordinated resorption by osteoclasts. The K-ASSAY Osteoclast Culture Kit / Bone Resorption Assay contains frozen mouse or rat osteoclast precursor cells (isolated from bone marrow), culture medium containing M-CSF and RANKL for growing osteoclasts. Tartrate-resistant acid phosphatase can be visualized with the optional K-ASSAY TRAP Kit (KT-008). 2 Rev. 100307

COMPONENTS Rat Osteoclast Precursor Cells, frozen Vial containing 2 x 10 6 cells 2 Washing Medium, alpha-mem 50 ml 1 Culture Medium, alpha-mem with M-CSF (50 ng/ml) and RANK Ligand (50 ng/ml) 25 ml 1 Mouse (BALB/C) Osteoclast Precursor Cells, frozen Vial containing 2 x 10 6 cells 1 Washing Medium, alpha-mem 50 ml 1 Culture Medium, alpha-mem with M-CSF (50 ng/ml) and RANK Ligand (50 ng/ml) 25 ml 1 CC-107 Rat Osteoclast Precursor Cells, V-1 Rat Osteoclast Precursor Cells, frozen Vial containing 2 x 10 6 cells 1 CC-109 Mouse Osteoclast Precursor Cells, V-1 Mouse (BALB/C) Osteoclast Precursor Cells, frozen Vial containing 2 x 10 6 cells 1 Storage Components Storage Conditions Shelf-Life Mouse or Rat Osteoclast Precursor Cells Liquid Nitrogen (preferred) See expiration date on box Washing Medium -20 C Freezer 6 months -80 C Freezer 1 year Culture Medium -20 C Freezer 6 months -80 C Freezer 1 year Materials required but not provided Distilled water Variable volume pipettes Microtiter plate, flat bottom Dentin Slices for Pit Formation Assay PRECAUTIONS 1. Read the instructions carefully before beginning the assay. 2. This kit is for research use only, not for human or diagnostic use. PROTOCOLS 1. Osteoclast Culture Procedure a. Quickly thaw osteoclast precursor cell vial in a 37 C water bath. b. Transfer thawed cells into a 15 ml centrifuge tube. Add 10 ml of Washing Medium and mix briefly. Centrifuge for 5 minutes at 4 C at 1,000 rpm. c. After removing the supernatant, add 10 ml of Washing Medium to the tube and mix briefly. Centrifuge for 5 minutes at 4 C at 1,000 rpm. 3 Rev. 100307

d. After removing the supernatant, add between 2.5 and 5 ml of Culture Medium (containing M-CSF, RANKL) into the tube to prepare a cell suspension. Dispense 100 µl of the suspension into each well of a 96-well plate (if you use 5 ml of the culture medium, half of the plate will be filled). i. If you want to see the osteoclast formation in a short period of time, make the cell density higher for the culture. ii. When the Pit Formation Assay is run, place a slice of the dentin slices into the well before starting the assay. Dentin Slices not included in kit. e. Change the culture medium (100 µl) every 3 to 4 days. i. Approximately 5 days after starting the culture, osteoclasts (formed from the fusion of several cells) will begin to form. ii. For an experiment on the control factor of osteoclast formation, add the control factor to the culture medium and culture in the wells for approximately 7 days. Proceed with TRAP staining (tartrate-resistant phosphatase staining) with optional TRAP Staining Kit (Cat. No. KT-008) and count the number of osteoclast cells. 2. Pit Formation Assays (requires Dentin Slices not included in kit) a. Pit Formation Assay (Staining Method): i. Disrupt cells (after being cultured on the dentin slice for 7 to 14 days) in 5 ml of 1M ammonia by sonication. ii. Remove dentin slice from the ammonia and stain with Mayer s (Gill) hematoxylin solution for 1 minute. iii. Wash with water and dry. iv. Measure the total area of the resorption pit formed by the osteoclast cells. b. Pit Formation Assay (SEM (scanning electron microscopy) Method): i. Process dentin slice as indicated in step 2.a. ii. Observe the dry section surface with scanning electron microscope and measure the number and area of resorption pits. If clear images of the pits are needed, SEM is recommended. 4 Rev. 100307

c. TRAP Staining is possible with the optional TRAP Staining Kit (Cat. No. KT- 008). FOR RESEARCH USE ONLY 5 Rev. 100307

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