Novel insights into Dhh signaling in antler chondrocyte proliferation and differentiation: Involvement of Foxa.

The desert hedgehog (Dhh) is crucial for spermatogenesis and Leydig cell differentiation, but little is known regarding its physiological function in cartilage. In this study, Dhh mRNA was abundant in antler chondrocytes, where it advanced cell proliferation concomitant with accelerated transition from the G1 to the S phase and induced elevation of the hypertrophic chondrocyte markers, Col X and Runx2. Silencing of Ptch1 resulted in appreciable Smo accumulation and enhanced rDhh stimulation of Smo, whose impediment by cyclopamine obscured the proliferative function of Dhh and alleviated its guidance of chondrocyte differentiation. Further analysis evidenced the noteworthy positive action of Smo in the bridging between Dhh and Gli transcription factors. Obstruction of Gli1 by GANT58 caused the failed stimulation of Col X and Runx2 by rDhh. Analogously, siRNA against Gli1-3 hindered chondrocyte differentiation in the context of rDhh. Simultaneously, Gli transcription factors mediated the regulation of Dhh on Foxa1, Foxa2, and Foxa3, whose knockdown impaired chondrocyte differentiation. Attenuation of Foxa antagonized the augmentation of Col X and Runx2 generated by rDhh. Collectively, Dhh signaling through its target Foxa appears to induce antler chondrocyte proliferation and differentiation.

Antler development and coupled osteoporosis in the skeleton of red deer Cervus elaphus: expression dynamics for regulatory and effector genes.

Antlers of deer display the fastest and most robust bone development in the animal kingdom. Deposition of the minerals in the cartilage preceding ossification is a specific feature of the developing antler. We have cloned 28 genes which are upregulated in the cartilaginous section (called mineralized cartilage) of the developing ("velvet") antler of red deer stags, compared to their levels in the fetal cartilage. Fifteen of these genes were further characterized by their expression pattern along the tissue zones (i.e., antler mesenchyme, precartilage, cartilage, bone), and by in situ hybridization of the gene activities at the cellular level. Expression dynamics of genes col1A1, col1A2, col3A1, ibsp, mgp, sparc, runx2, and osteocalcin were monitored and compared in the ossified part of the velvet antler and in the skeleton (in ribs and vertebrae). Expression levels of these genes in the ossified part of the velvet antler exceeded the skeletal levels 10-30-fold or more. Gene expression and comparative sequence analyses of cDNAs and the cognate 5' cis-regulatory regions in deer, cattle, and human suggested that the genes runx2 and osx have a master regulatory role. GC-MS metabolite analyses of glucose, phosphate, ethanolamine-phosphate, and hydroxyproline utilizations confirmed the high activity of mineralization genes in governing the flow of the minerals from the skeleton to the antler bone. Gene expression patterns and quantitative metabolite data for the robust bone development in the antler are discussed in an integrated manner. We also discuss the potential implication of our findings on the deer genes in human osteoporosis research.

Stem cells responsible for deer antler regeneration are unable to recapitulate the process of first antler development-revealed through intradermal and subcutaneous tissue transplantation.

Antlers offer a unique model for the study of whether regeneration recapitulates development in a mammalian organ. Research, to date, supports the full recapitulation in antler, but a recent report that subcutaneously transplanted (ST) pedicle periosteum (PP) failed to induce that ectopic antler formation could argue against recapitulation, as antlerogenic periosteum (AP) can readily do so. However, it was not clear in that study whether the result was caused by inability of the PP to interact with the skin or owing to failure to create the required close contact to it. This study was designed to clarify this uncertainty by adopting intradermal transplantation (IT) to achieve the required close contact without the need for significant mass expansion. The results showed that IT of 1/8 of the original AP mass or more was sufficient for antler induction, whereas ST of 1/4-AP or less could not do so within 2 years. The minimum amount of AP required for antler induction using the IT approach was somewhere between 1/8 and 1/12-AP (<30 mg). The results further demonstrated that IT of 62-84 mg PP failed to induce ectopic antler formation, even if the PP had fused with the surrounding skin. Because this mass of PP was 2-3 times the minimum amount of AP required for antler induction, we conclude that PP does not recapitulate AP in induction of ectopic antler development. It is likely that PP has been restricted for antler regeneration and lost the potential to initiate antler development.

Testosterone, but not IGF-1, LH, prolactin or cortisol, may serve as antler-stimulating hormone in red deer stags (Cervus elaphus).

The role of androgens and insulin-like growth factor 1 (IGF-1) in antler growth has been disputed. We predicted that the secretory of IGF-1 may be associated with an acceleration of body growth rather than with antler growth. Furthermore we anticipated a relationship between the increase of testosterone and the progress of antler growth. If IGF-1 is involved in the stimulation of antler growth, this should be more obvious in young than in mature stags. Eight two-year-old red deer stags (Cervus elaphus), and twelve adult red deer stags were blood sampled and the length of their velvet antlers was measured in one-week intervals during the period of antler growth. Concentrations of testosterone, cortisol, IGF-1, luteinizing hormone (LH), and prolactin were determined in plasma by enzyme immunoassay or radioimmunoassay. Antler growth per day was primarily dependent on changes in testosterone concentration per day in both groups of stags. As expected, only in two-year-old stags we detected a possible role of IGF-1 in the antler growth regulation, but that was not in agreement with previously published studies. Nevertheless, this effect was still utilized in interaction with testosterone. In addition to total antler length, only concentrations of testosterone and LH were significantly higher in adult males in comparison to two-year-old males. Our present results lead us to conclude that it is not IGF-1 but testosterone which is responsible for the intensity of antler growth in subadult and adult red deer stags.

Identification of differentially expressed genes in the developing antler of red deer Cervus elaphus.

Understanding the molecular mechanisms underlying bone development is a fundamental and fascinating problem in developmental biology, with significant medical implications. Here, we have identified the expression patterns for 36 genes that were characteristic or dominant in the consecutive cell differentiation zones (mesenchyme, precartilage, cartilage) of the tip section of the developing velvet antler of red deer Cervus elaphus. Two major functional groups of these genes clearly outlined: six genes linked to high metabolic demand and other five to tumor biology. Our study demonstrates the advantages of the antler as a source of mesenchymal markers, for distinguishing precartilage and cartilage by different gene expression patterns and for identifying genes involved in the robust bone development, a striking feature of the growing antler. Putative roles for "antler" genes that encode alpha-tropomyosine (tpm1), transgelin (tagln), annexin 2 (anxa2), phosphatidylethanolamine-binding protein (pebp) and apolipoprotein D (apoD) in intense but still controlled tissue proliferation are discussed.

Expression of PTHrP and the PTH/PTHrP receptor in growing red deer antler.

Antler growth is highly co-ordinated, so that trabecular bone and antler skin (velvet) develop together, at a rapid rate and in a manner reminiscent of their development in the fetus. Parathyroid hormone-related peptide (PTHrP) is expressed in both bone and skin, and is therefore a candidate to effect co-ordination between these tissues. The aim of this study was to localize the expression of PTHrP and its principal receptor, the parathyroid hormone/parathyroid hormone-related peptide receptor (PTH/PTHrPR), in antler ("spiker") of one-year-old red deer. Using immunohistochemistry and in situ hybridization, intense and overlapping expression of PTHrP and its receptor was seen in developing osseocartilaginous structures and in the underlying layers of velvet epidermis. PTHrP was located on both the cell surface and within the nuclei. Our results strongly suggest that PTHrP, acting via the PTH/PTHrPR and possibly other intracrine mechanisms, plays a central role in the co-ordinated regulation of cell division and differentiation of developing antler bone and skin.

Bone turnover associated with antler growth in red deer (Cervus elaphus).

Although it is known that skeletal bone depletion occurs during antler growth in deer, it is not clear whether repletion of the skeleton takes place before or after completion of antler development. This study attempted to correlate repeated scanning electron microscopic measures of ilium and rib bone porosity from six approximately 2-monthly biopsy samples (using back-scattered imaging) and biochemical markers of bone turnover (serum hydroxyproline and osteocalcin concentrations) taken for 11 months with antler growth in six red deer stags. No changes were detected in ilium samples but changes in porosity of rib bones and an elevation of the biochemical markers indicated that skeletal depletion occurred during the antler growth period. However, the decrease in rib bone porosity and decline in markers of bone turnover took place before completion of antler growth, indicating that a considerable amount of skeletal repletion could have occurred whilst antlers were also undergoing bone accretion. This latter finding extends the current view of antler growth being accompanied by a form of reversible osteoporosis in the skeleton by showing that there is a period when the antlers and skeleton are both undergoing net bone formation.

Morfometría, patrones de crecimiento y ganancia de peso de venados cola blanca (Odocoileus virginianus) en cautiverio en Durango y Toluca, México / Morphometrics, growth and weight gain patterns in White-Tailed deer (Odocoileus virginianus) in captivity in Mexico

Las tasas de crecimiento, ganancias diarias de peso y medidas corporales fueron estudiadas en venados cola blanca (O. virginianus) (n = 35) en Durango y Toluca, México, de 1989 a 1994. Los cervatillos pesaron al nacer 2.3 kg en promedio (ee = 0.873, n = 14), tienen una ganancia de peso promedio de 225.5 g/día (ee = 25.7, n = 4) y de 107.0 g/día (ee = 38.4, n = 7), el promedio de días de lactancia fue de 112.2 y 88.5 días y el peso promedio al destete fue de 14.5 y 12.6 kg para cervatillos en lactancia natural y artificial, respectivamente. Se notifican las medidas corporales tomadas semanalmente, desde el nacimiento al destete; los largos total del cuerpo, de las patas traseras, de las patas delanteras y de las orejas de cervatillos en lactancia artificial. Los machos adultos (n = 10) continúan su crecimiento hasta después de los cinco años de edad y las hembras (n = 11) estabilizan su peso al tercer año de edad. Se discuten los efectos de la dieta, productividad primaria del hábitat y variaciones entre subespecies como factores reguladores del crecimiento. Los patrones de crecimiento de esta especie en México son similares a lo descrito en Estados Unidos de América y Canadá, para la familia Cervidae y para otros ungulados silvestres y domésticos de climas templados

Detection of growth factors and proto-oncogene mRNA in the growing tip of red deer (Cervus elaphus) antler using reverse-transcriptase polymerase chain reaction (RT-PCR).

Deer antler is a unique mammalian organ that has an annual cycle of regeneration. The antler grows very rapidly from the tip at up to 1 cm/day in red deer for a 90- to 120-day period. It is hypothesised that locally produced growth factors are required to control and stimulate this growth. The tip of the growing antler from animals whose antlers had been growing for 30, 60, or 90 days was dissected into four zones: epidermis/dermis, reserve mesenchyme, precartilaginous, and cartilaginous. Total RNA was extracted, and the presence of various growth factors and proto-oncogenes was detected using RT-PCR, IGF-I, IGF-II, TGF beta 1, TGF beta 2, c-fos, c-myc, and beta-actin were all present as single bands of the expected molecular weight in the four zones of the antler at each stage of growth. There were higher levels of IGF-I, TGF beta 2, and c-myc relative to beta-actin in the epidermis/dermis layer than in the other three zones. There were no differences in the expression of any of the genes between the three stages of growth. The presence of TGF beta 3 cannot be confirmed since multiple bands were seen in all antler tissues. A single band of the expected size for TGF alpha was seen only in the epidermal/dermal layer of the antler, with multiple bands of different molecular weight being detected in the other zones of the antler. This work has demonstrated the presence of multiple growth factors in the growing deer antler and supports the hypothesis that paracrine/autocrine stimulation is important for regulating antler growth.

Deer herd health and production profiling in New Zealand. 2. Preliminary results.

A 2 yr observational study of 15 commercial red deer farms is being conducted in New Zealand and statistical analysis initiated. Preliminary results for weaner deer growth, reproduction and deer mortality data are presented. Multivariable statistical analyses are used to identify risk factors for these various outcomes. Factors associated with yearling hind conception status were included in a putative path diagram and logistic regression was used to identify important factors.

Characteristics of male fallow deer muscle at a time of sex-related muscle growth.

Muscle characteristics of male fallow deer undergoing neck muscle enlargement as the mating season (rut) approached were studied. Five commercially-raised males were slaughtered prerut and five were slaughtered 11 weeks later, just before the rut began. During this period, increases in individual muscle weight were not the same: two of the three neck muscles studied grew more rapidly than the average, whereas the back and two hind leg muscles grew more slowly. The splenius, the neck muscle that grew the most apparently in response to a rise in plasma testosterone, was studied. Cryosections were cut and stained for myofibrillar ATPase so that the muscle fiber classes--slow oxidative (type I), fast oxidative-glycolytic (type IIA) and fast glycolytic (type IIB)--could be distinguished. The IIB class was absent from the splenius and the occurrence of I and IIA fibers did not change during the period of splenius growth. However, the splenius of fallow deer increased in activity of NADH-tetrazolium oxidoreductase at the fiber peripheries as the rut approached. Further, fiber areas increased markedly during the period of growth, with type I fibers doubling in area and type IIA nearly trebling. Thus, the endocrinal and/or neural changes associated with the rut differentially affected these fiber types, and since type IIA fibers outnumbered type I by nearly 2 to 1, muscle enlargement is clearly dominated by the former class. Fiber areas were normally distributed for both fiber types, prerut and at the start of the rut, and coefficients of variation were similar. These results suggest that all fibers within a type are equally liable to grow during the growth period.

Endocrine control of antler growth in red deer stags.

Observations of body weight, testis size, antler status, plasma testosterone and prolactin were made on 12 red deer stags during their first 2 years of life. Six of the stags were fed to appetite throughout the study (Group A) and 6 were fed a 70% restricted diet during each winter (Group B). In addition 6 of the stags , 3 from each group, were studied in more detail; LH and testosterone were measured either after a single injection of LH-RH or in samples taken at frequent intervals over a period of 8 or 24 h. During the study the stags became sexually mature, developed first their pedicles and then antlers and showed at least one complete cycle of casting and regrowth of the antlers . The stags in Group A developed their testes and pedicles about 2 months earlier than did those in Group B. Pedicle initiation was associated with increasing plasma testosterone levels in response to changes in LH secretion, and antler development occurred when testosterone levels were low or decreasing. Cleaning of the velvet was associated with high levels of plasma testosterone. Antler casting occurred when plasma testosterone concentrations were low or undetectable and prolactin levels were high or increasing. The relationship between LH and testosterone varied during the study; in spring when the testes and antlers were growing, relatively high levels of LH were associated with only small peaks of testosterone, yet in summer, when antler growth was complete and the antlers were clean of velvet, low LH concentrations were associated with large peaks of testosterone.