Abstract
Even a casual pass through the great halls of mammals in the world’s natural history museums highlights the wide diversity of skeletal proportions that allow us to distinguish between species even when reduced to their calcified components. Similarly each individual is comprised of a variety of bones of differing lengths. The largest contribution to the lengthening of a skeletal element, and to the differential elongation of elements, comes from a dramatic increase in the volume of hypertrophic chondrocytes in the growth plate as they undergo terminal differentiation1–7. Despite this recognized importance, the mechanisms of chondrocyte volume enlargement have remained a mystery8–11. Here we use quantitative phase microscopy12 to show that chondrocytes undergo three distinct phases of volume increase, including a phase of massive cell swelling in which the cellular dry mass is significantly diluted. In light of the tight fluid regulatory mechanisms known to control volume in many cell types13, this stands as a remarkable mechanism for increasing cell size and regulating growth rate. It is, however, the duration of the final phase of volume enlargement by proportional dry mass increase at low density that varies most between rapidly and slowly elongating growth plates. Moreover, we find that this third phase is locally regulated through an Insulin-like Growth Factor-dependent mechanism. This study provides a framework for understanding how skeletal size is regulated and for exploring how cells sense, modify, and establish a volume set point.
Each of the long bones initially forms in the embryo as a similarly sized cartilage rudiment that only subsequently undergoes differential regulation of growth. The elongation of a skeletal element occurs at the growth plate14,15, each consisting of three distinct zones: resting round chondrocytes near the end of an element give rise to clonal columns of flattened proliferating chondrocytes that then terminally differentiate into hypertrophic chondrocytes nearest the bony center of an element. While multiple cellular parameters contribute to lengthening of skeletal elements - including proliferation, matrix deposition, and hypertrophic cell enlargement - the greatest contribution to growth rate in mammals is due to the massive volume enlargement of hypertrophic chondrocytes expanding the skeletal tissue in the direction of longitudinal growth within laterally restricting matrix channels1–3. In addition to being the largest contributor to the elongation rate of a given skeletal element, this parameter is largely responsible for the difference in growth rates between different skeletal elements within an individual, between homologous elements in different species, and within a single element as an animal ages4–7. Surprisingly, however, given its critical importance in determining the growth rate of each bone and the overall stature of the individual, the mechanism is poorly understood. It even remains unclear whether hypertrophic chondrocyte volume increases by true hypertrophy, maintaining constant density during growth through an increase in macromolecules and organelles, or by cell swelling via disproportionate fluid uptake which is ordinarily a hallmark of disease13.
To determine whether hypertrophic chondrocytes enlarge by cellular hypertrophy and/or swelling, we applied methods of diffraction phase microscopy to measure the dry mass of individual unstained live cells dissociated from growth plate cartilage. (Fig. 1a; Supplementary Methods)16. Together with volume information about the sample, calculated here based on a well-supported spherical approximation for dissociated chondrocytes (Supplementary Methods), this allows the calculation of dry mass density. Diffraction phase microscopy measurements of a variety of cell types consistently reflect a “normal” dry mass density for healthy living cells at approximately 0.182 pg/fl in agreement with the concentration of cytoplasm previously determined by index matching in human oral epithelial cells17. This includes maturing megakaryocytes that reach volumes comparable to the largest hypertrophic chondrocytes and ten-times the average somatic cell volume (Supplementary Fig. S1).
In contrast, analysis of chondrocytes from the rapidly elongating mouse proximal tibia reveals that there are three distinct phases of hypertrophic cell enlargement. 1) An initial increase of about 3-fold from approximately 600 fl to 2000 fl is characterized by true hypertrophy - a proportionate increase in dry mass production and fluid uptake thus maintaining the normal dry mass density at 0.183 pg/fl (Fig. 1b, c). 2) A second phase where a 4-fold enlargement from about 2000 fl to 8000 fl is characterized by cell swelling. Volume increases at a rate disproportionate to the continuing rate of dry mass production resulting in a dramatic dilution of dry mass density to approximately 0.07 pg/fl (Fig. 1c). 3) At volumes larger than 8000 fl, the dry mass density once again stabilizes, and cells continue to enlarge another 2-fold to about 14,000 fl by proportionately increasing dry mass and fluid volume at this lower density (Fig. 1d). Swelling in Phase 2 allows cells to reach volumes two to three times greater in Phase 3 than if they relied entirely on the proportionate increase in dry mass at high density (Fig. 1b, linear regression).
To verify that this decrease in density is characteristic of hypertrophic differentiation, we imaged a subset of the small high-density cells and large low-density cells using regularized tomographic phase microscopy to generate a refractive index map of dry mass density in three-dimensions (Supplementary Methods). This independent approach confirms that the largest cells reduce their dry mass density by approximately 60%, and moreover indicates that dry mass is low throughout the cytoplasm with a slightly higher density ring around the nucleus (Fig. 1e, f; Supplementary Fig. S14).
Understanding the cellular process by which hypertrophic cells enlarge provides a framework for considering how that process is modulated to achieve differential growth of individual elements within a species and of homologous elements between species. In contrast to the large hypertrophic chondrocytes of the rapidly elongating proximal tibia, the slowly elongating proximal radius has much smaller hypertrophic chondrocytes1. We find that these cells go through Phase 1 and enter Phase 2 similar to the cells of the proximal tibia, reaching a volume of approximately 5,000 fl. However, they truncate the remainder of Phase 2 after dilution of dry mass density to approximately 0.10 pg/fl and completely eliminate Phase 3 (Fig. 2a).
We next compared growth plates of the mouse to those of the jerboa, a small bipedal rodent with greatly elongated hindlimbs. In particular, the metatarsals of the feet rapidly elongate during early postnatal development to approximately 2.5 times the relative proportion of mouse metatarsals18. The mouse distal metatarsal growth plate is intermediate in its growth rate and hypertrophic chondrocyte size relative to the proximal tibia and radius (Fig. 2b; Supplementary Fig. S2). While other aspects of the jerboa distal metatarsal growth plate are also altered, including the total cell number in each zone (Supplementary Fig. S3), the height of individual hypertrophic chondrocytes is increased by 58% compared to those in the homologous growth plate of the mouse suggesting a significant contribution of hypertrophic chondrocyte volume to the increased rate of growth of this element (Fig. 2b, e, f). In contrast, the jerboa tibia hypertrophic chondrocytes are only slightly larger than their counterparts in the mouse (Fig. 2b, c, d). Unlike the metatarsals, the metacarpals of the jerboa forelimb, as well as other bones of the forelimb, are similar in size and proportions to those of the mouse with hypertrophic chondrocytes of comparable size (Fig. 2b).
The hypertrophic chondrocytes of the jerboa proximal tibia show very similar growth properties to those of the mouse when examined by diffraction phase microscopy, including all three phases of volume enlargement (Supplementary Fig. S4). However, there is a striking difference between the metatarsal chondrocytes of the two species. Mouse metatarsal hypertrophic chondrocytes are indeed intermediate in size between the proximal radius and proximal tibia, reaching a maximum volume of about 8000 fl by completing Phases 1 and 2 and truncating Phase 3 (Fig. 2g). Hypertrophic chondrocytes of the jerboa metatarsals increase almost 40-fold from their initial volume to approximately 23,000 fl, greater than the volume of tibia chondrocytes in either species (Fig. 2h). This is accomplished by following the same tri-phasic growth trajectory common to chondrocytes of other growth plates and then extending Phase 3 to reach a maximal volume by continued proportionate increase in dry mass and fluid volume at low dry mass density.
Little is known about the molecular mechanisms that control chondrocyte enlargement, or the regulation of final cell size, since few of the mutants affecting skeletal development have been examined for size of individual hypertrophic chondrocytes. An intriguing exception is the null mutation of the gene encoding Insulin-like Growth Factor 1 (Igf1)19. Igf1 functions in a variety of target tissues to promote protein synthesis and cell growth19,20 and is strongly expressed in both proliferating and pre-hypertrophic chondrocytes. Igf1-deficient mice are 35% smaller than controls but have the same number of hypertrophic chondrocytes, though each cell is 30% shorter in the direction of elongation, a finding we confirmed in mice where the floxed Igf1tm1Dlr allele21 was conditionally deleted from the hindlimb using HoxB6-Cre22 (Fig. 3a–c). It is additionally intriguing to note that there is no distinction between the heights of chondrocytes in the proximal tibia and distal metatarsal of this mutant (Fig. 3c) indicating that Igf1 may play an important role in the establishment of growth plate dependent cell size. While this effect could be modulated by any member of the Igf1 signaling pathway, evidence suggests a possible role for the receptor, Igf1R, that maintains higher levels of expression over time in growth plates that continue to elongate at faster rates in maturing mice23.
We employed diffraction phase microscopy to determine which phase(s) of volume enlargement are affected by Igf1. Igf1-deficient hypertrophic chondrocytes undergo normal Phase 1 and Phase 2 of enlargement, reaching approximately 7000 fl largely by cell swelling, but do not progress to Phase 3 and thus fail to further double their volume by the continued production of dry mass at low density (Fig. 3d–f). Taken together, our results indicate that there are three distinct phases of chondrocyte hypertrophy, and it is regulation of the Igf1-dependent third phase that is responsible for much of the variation in skeletal elongation rate.
Finally, previous studies of the neonatal bat and mouse forelimb suggested that the entire hypertrophic zone of each growth plate turns over once in about 24 hours regardless of the maximum volume attained by individual chondrocytes, the number of hypertrophic chondrocytes, or rate of growth plate elongation7. This suggests that growth plates elongating at different rates adjust the rate of cell volume increase to fall within a 24-hour lifespan constraint. To assess the pace of cellular maturation and enlargement, we marked proliferating chondrocytes with BrdU and followed the progression of the first labeled cells to emerge into the postmitotic hypertrophic columns onward to the chondro-osseous junction (Supplementary Fig. S5). We find that the rate of cell height increase in both growth plates is extremely rapid, more than tripling the height of proximal tibia chondrocytes within approximately 12 hours (Fig. 4a). Once cells reach their average final height, with a steeper slope in the larger cells of the tibia, they remain at this terminal size in the hypertrophic growth columns for an additional 12 hours before turnover at the chondro-osseous junction.
Through coordination of this multiphase process, cell swelling allows chondrocytes to enlarge extraordinarily rapidly while presumably lowering the energetic cost of growth, and volumes are subsequently amplified in the most rapidly elongating skeletal elements by the continued Igf1-dependent production of mass. This unique mechanism of volume enlargement suggests that chondrocyte hypertrophy will serve as a valuable model for cell volume homeostasis, in addition to our findings that provide insight into skeletal morphogenesis and evolution.
Full Methods
Animals
CD-1 was chosen as the wild type mouse strain for this study. Igf1tm1Dlr conditional mice21 and HoxB6-Cre transgenic mice22 were previously described. Jerboas were housed and reared as previously described24. All animal protocols were approved by the Harvard Medical Area Standing Committee on Animals.
Sectioning and histology
Dissected skeletal elements were fixed overnight at 4°C in 4% paraformaldehyde and then carried through a graded series of ethanol dehydration washes before transition through xylenes and into paraffin wax. Sections were cut at 10–12 μm thickness and stained with hematoxylin and eosine. Average maximum cell heights were measured in the axis of linear growth through the lacunae surrounding the largest cells with a clear nuclear profile from digital images of the hypertrophic zone and averaged across at least 4 sections from at least 3 individuals. Bromodeoxyuridine (100 mg/kg) or oxytetracycline hydrochloride (20 mg/kg) was injected into the peritoneum of postnatal day 5 mice before harvest. BrdU was detected using a rat anti BrdU (AbD Serotech) followed by goat anti-rat Alexa594 (Invitrogen) in paraffin sections. Oxytetracycline was detected by fluorescence in bisected skeletal elements.
Chondrocyte and megakaryocyte isolation
Postnatal day 5 animals were chosen for this study because the tibia and metatarsal growth plates are rapidly elongating in both species, but the metatarsal epiphysis (secondary ossification center) has not yet formed. While the epiphysis of the metatarsal forms by P7 in the mouse, it appears later in the jerboa (Fig. S3). Since the hypertrophic chondrocytes reside in a small domain nearest the chondro-osseous junction, we enriched for these cells by using a razor blade to remove a majority of the cartilage containing resting and proliferative chondrocytes leaving the cells closest to the chondro-osseous junction and a small amount of the adjacent trabecular bone. Growth plates were bisected longitudinally and incubated for 45 minutes at 37°C in 2 mg/ml Collagenase D (Roche) in DMEM/F12 (Invitrogen, 290–330 mOsm) plus 10% fetal calf serum. After the initial incubation, the bone collar, trabecular bone, and loosened connective tissues were manually removed with forceps, and the remaining cartilage fragments were transferred to a fresh dish of collagenase digestion media. Cells were incubated for an additional 2–3 hours with occasional swirling until cells mostly dissociated from the surrounding matrix. Dissociated chondrocytes were transferred to 35 mm dishes with a 14 mm diameter, 1.5-thickness glass bottom (MatTek) and imaged immediately. The largest hypertrophic chondrocytes are a small population of the most mature cells, therefore we further enriched for this population in our data analysis by scanning for fields of view containing the largest cells in the dish and quantified all of the intact spherical neighbors.
There has been a longstanding discussion in the literature regarding the extracellular osmolarity of chondrocytes, primarily in the articular cartilage9,10,25,26. Much of this data is based on the theoretical ionic environment in association with charged glycosaminoglycans according to the Donnan-Gibbs equilibrium, though to our knowledge the extracellular osmolarity of growth plate cartilage has not been directly measured. While serum osmolarity is approximately 280 mOsm, the osmolarity in association with cartilage may be upwards of 400 mOsm. To address the possibility that the swelling we observe in chondrocytes at larger volumes may be the response to media of low osmolarity, we repeated the diffraction phase microscopy measurements in mouse proximal tibia growth plates dissociated in 424 mOsm DMEM/F12 raised with sucrose. Media osmolarity was measured using the Vapro Model 5600 (Wescor, Inc). We find the same three phases, including the phase of cell swelling, indicating this is an inherent property of growth plate chondrocytes and not the passive response to an abnormal osmotic environment (Fig. S6). We presume that the 4 hours from dissection to imaging is enough time for volume regulatory mechanisms to compensate for any response to osmotic stress that may have occurred. Indeed, 4-D confocal imaging of in situ porcine articular chondrocytes after osmotic stress shows a mean recovery rate of 4.1%±1.8%/min with 96% volume recovery after about 12 minutes27.
Fetal megakaryocytes were isolated from embryonic day 14.5 mouse livers according to previously published protocols28,29 or generously donated by Dr. Annouck Luyten and Dr. Ramesh Shivdasani. Cells were imaged by DPM one day after harvest or at maturity after five days in culture.
Supplementary Material
Acknowledgments
We would like to thank T.J. Mitchison, C.E. Farnum, and members of the Developmental Bone Morphogenesis program project grant (NIH) for helpful discussions. We also thank the Nikon Imaging Center at Harvard Medical School for technical support, A. Luyten and R. Shivdasani for providing mouse megakaryocytes, and P. Ramirez for jerboa care. This work was supported by National Institutes of Health (NIH) grants P01DK056246 to C.J.T, R01GM026875 to M.W.K., and by NIH grant P41RR02594, National Science Foundation (NSF) grant DBI0754339 and support from the Hamamatsu Corporation to R.R.D.
Footnotes
K.L.C. and S.O. conceived of the project and carried out the majority of the experiments. Y.S. and D.R. carried out critical spectroscopic experiments validating the primary approaches taken. C.J.T. and M.W.K. supervised the project. K.L.C., S.O., M.W.K. and C.J.T. wrote the manuscript.
The authors declare no competing financial interests.
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