Osteoclast-derived IGF1 induces RANKL production in osteocytes and contributes to pagetic lesion formation
Kazuaki Miyagawa, Hirofumi Tenshin, Patrick L. Mulcrone, Jesus Delgado-Calle, Mark A. Subler, Jolene J. Windle, John M. Chirgwin, G. David Roodman, Noriyoshi Kurihara
Kazuaki Miyagawa, Hirofumi Tenshin, Patrick L. Mulcrone, Jesus Delgado-Calle, Mark A. Subler, Jolene J. Windle, John M. Chirgwin, G. David Roodman, Noriyoshi Kurihara
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Research Article Bone biology Endocrinology

Osteoclast-derived IGF1 induces RANKL production in osteocytes and contributes to pagetic lesion formation

Abstract

We previously reported that measles virus nucleocapsid protein (MVNP) expression in osteoclasts (OCLs) of patients with Paget disease (PD) or targeted to the OCL lineage in MVNP-transgenic mice (MVNP mice) increases IGF1 production in osteoclasts (OCL-IGF1) and leads to development of PD OCLs and pagetic bone lesions (PDLs). Conditional deletion of Igf1 in OCLs of MVNP mice fully blocked development of PDLs. In this study, we examined whether osteocytes (OCys), key regulators of normal bone remodeling, contribute to PD. OCys in PDLs of patients and of MVNP mice expressed less sclerostin, and had increased RANKL expression compared with OCys in bones from WT mice or normal patients. To test whether increased OCL-IGF1 is sufficient to induce PDLs and PD phenotypes, we generated TRAP-Igf1 (T-Igf1) transgenic mice to determine whether increased IGF1 expression in the absence of MVNP in OCLs is sufficient to induce PDLs and pagetic OCLs. We found that T-Igf1 mice at 16 months of age developed PD OCLs, PDLs, and OCys, with decreased sclerostin and increased RANKL, similar to MVNP mice. Thus, pagetic phenotypes could be induced by OCLs expressing increased IGF1. OCL-IGF1 in turn increased RANKL production in OCys to induce PD OCLs and PDLs.

Authors

Kazuaki Miyagawa, Hirofumi Tenshin, Patrick L. Mulcrone, Jesus Delgado-Calle, Mark A. Subler, Jolene J. Windle, John M. Chirgwin, G. David Roodman, Noriyoshi Kurihara

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Figure 3

Characterization of primary OCys from WT and MVNP mice.

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Characterization of primary OCys from WT and MVNP mice. (A) Sost and Igf...
(A) Sost and Igf1 mRNAs: Primary OCys were isolated form long bones from 20-month-old WT and MVNP mice by sequential digestion with collagenase as described in Methods. Fractions 6–9 were used. RNA was extracted from 2 × 106 cells from 4 individual WT or MVNP mice and analyzed by TaqMan PCR. Data for Sost and Igf1 are the mean ± SEM (3 technical replicates from the mice) analyzed using the Mann-Whitney U test in A and C. (B) Sclerostin and DMPI protein: OCys were fixed, stained with anti-sclerostin or -DMP1 antibody and fluorescent secondary antibody conjugates, and examined by immunofluorescence. Scale bars: 10 μm. (C) The pixel intensity of positive cells was measured using a laser confocal microscope. Results shown relative pixel intensity of cells in 30 random cells from 3 wells, mean ± SEM from 1 average value per sample and analyzed using a 1-way ANOVA with Tukey’s test. The experiment was performed 3 times using different biological replicates with similar results.