Expression on outer membranes of mannose residues, which are involved in osteoclast formation via cellular fusion events

T Kurachi,I Morita,T Oki,T Ueki,K Sakaguchi,S Enomoto,S Murota

doi:10.1016/s0021-9258(17)32479-1

T Kurachi, I Morita + Show 5 more

Open Access

https://doi.org/10.1016/s0021-9258(17)32479-1

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Abstract

Osteoclast, the bone-resorbing cell, is formed from hematopoietic precursors via cell-cell fusion. To evaluate the possibility that under certain specific conditions mannose residues may be expressed on the mammalian cell surface, we examined the action of pradimicin derivatives, which bind specific sugars such as the mannose residue, on the formation of osteoclast induced in the coculture of mouse spleen cells with mouse stromal cells, a process in which cell-cell fusion is involved. Osteoclast formation was inhibited by treatment of this coculture system with pradimicin at the later stage (day 4-7), and this inhibition was specifically abrogated by mannose-rich yeast mannan. During the 8-day cocultivation, osteoclast formation was blocked by the pradimicin on days 6 and 7, when mononuclear preosteoclasts fused into multinucleated osteoclasts. With an interactive laser cytometer ACAS570, fluorescein isothiocyanate-labeled pradimicin was observed to bind osteoclast progenitors at the fusion stage and to have no binding affinity for osteoclast progenitors at the early stage (day 0-3) or for osteoclasts, which were formed after performing fusion between mononuclear preosteoclasts. These results suggest that mannose residues were expressed on outer membranes of monocytes under pathophysiological conditions and that they were involved in the osteoclast formation via cellular membrane fusion events.

Highlights

To study mechanismsof such eventsas the entryof enveloped viruses into host cells, virally induced cell-cell fusion, which leads to cell death, and the formation of giant cells during inflammatory reactions
MM sodium tartrate as previously described (14).tartrate-resistant acid phosphatase (TRACP)-positive cells with three or more nuclei were counted as multinucleated cells (MNCs)
There- TRACP-positive MNC formation throughinteraction with fore, we studied what kinds of hexoses or amino sugars were mannose residues on osteoclast progenitors

Summary

EXPERIMENTAL PROCEDURES

Cell Lines and Culture Conditions-Mouse stromal cell line TMS-14 was isolated and cloned from the bone marrow according to the method established in this laboratory (13).Murine spleen cells were prepared. The abbreviations used are: HIV, human immunodeficiency virus; by the modified method previously described (13).The purified spleen. TRACP, tartrate-resistant acid phosphatase; MNCs, multinucleated Urografin (ScheringAG, Germany) were seeded onto the TMS-14 strocells; MOPS, 3-(N-morpholino)propanesulfonicacid. The cultures were maintainefdor 8 days with medium change every 3 days with or without pradimicin and/or mannose-rich yeast mannan (Sigma). The cultures were dried and stained for tartrate-resistant acid phosphatase (TRACP) by incubating them in0.1 M sodium acetate buffer (p5H.0)containing naphtholAS-BI phosphoric acid sodium salt and fast redITR salt in thepresence of 10. MM sodium tartrate as previously described (14).TRACP-positive cells with three or more nuclei were counted as multinucleated cells (MNCs)

DAY aEdg

TRACP POSITIVE MONONUCLEAR CELL FORMATION

RESULTS

ICONTROL IPRADlMlClN