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Cd90.2 beads

Manufactured by Miltenyi Biotec
Sourced in United States

CD90.2 beads are a type of magnetic separation beads manufactured by Miltenyi Biotec. They are used to isolate and enrich CD90.2-positive cells from various biological samples. The beads are designed to bind to the CD90.2 surface marker, allowing for the separation and purification of the target cell population.

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2 protocols using cd90.2 beads

1

Culturing THY-1+ Germ Cells from Murine Testes

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THY‐1+ germ cell cultures were established as described previously.8 Briefly, male C57 LacZ pups (5‐8 days post‐partum) were sacrificed and testes were digested using Trypsin‐EDTA (Gibco, USA). Cells were magnetically sorted using CD90.2 beads (Miltenyi, USA) and plated onto Sandos inbred mouse (SIM)–derived 6‐thioguanine‐resistant and ouabain‐resistant (STO) feeders (SNL76/7, ATCC). Germ cell cultures were maintained in a humidified atmosphere at 37°C contains 5% CO2 with Mouse serum‐free media (mSFM) with 20 ng/mL recombinant human GDNF (R&D, USA), 150 ng/mL recombinant rat GFRα1 (R&D) and 1 ng/mL recombinant human FGF2 (Corning, USA). Other reagents were used as indicated: recombinant human FGF9 (R&D), SB203580, GW788388 and Tofacitinib citrate (all from MedChemExpress, USA). Germ cell counts were determined with a hemocytometer. Feeder cells were identified and discounted from counts based on morphology.22 SSC number was calculated using the following formula, adapted from reference 4: SSCgrowth=CellsharvestedCellsseeded×Colonies105cellstransplanted
Here, ‘cells seeded’ indicates the number of cultured THY‐1+ germ cells seeded at the beginning of each time period and ‘cells harvested’ is the cell count at the end. ‘Colonies’ indicates the number of distinct colonies counted per testis and is divided by the number of cultured THY‐1+ germ cells transplanted per testis.
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2

Hematopoietic Cell Reconstitution Assay

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Bone marrow cells were harvested from WT CD45.1 or Tracf/f E8Icre CD45.2 donors and depleted of T cell precursors using CD90.2 beads (Miltenyi) according to manufacturer’s instructions. An equal mix of 5×106 total cells from WT CD45.1 and Tracf/f E8Icre CD45.2 donors was intravenously injected into sub-lethally irradiated (6 Gy) Rag1−/− hosts. Mice were analyzed 12–16 weeks after reconstitution.
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