The insulin sensitiser metformin regulates chicken Sertoli and germ cell populations.

Metformin, an insulin sensitiser from the biguanide family of molecules, is used for the treatment of insulin resistance in type 2 diabetes individuals. It increases peripheral glucose uptake and may reduce food intake. Based on the tight link between metabolism and fertility, we investigated the role of metformin on testicular function using in vitro culture of Sertoli cells and seminiferous tubules, complemented by in vivo data obtained following metformin administration to prepubertal chickens. In vitro, metformin treatment reduced Sertoli cell proliferation without inducing apoptosis and morphological changes. The metabolism of Sertoli cells was affected because lactate secretion by Sertoli cells increased approximately twofold and intracellular free ATP was negatively impacted. Two important pathways regulating proliferation and metabolism in Sertoli cells were assayed. Metformin exposure was not associated with an increased phosphorylation of AKT or ERK. There was a 90% reduction in the proportion of proliferating germ cells after a 96-h exposure of seminiferous tubule cultures to metformin. In vivo, 6-week-old chickens treated with metformin for 3 weeks exhibited reduced testicular weight and a 50% decrease in testosterone levels. The expression of a marker of undifferentiated germ cells was unchanged in contrast to the decrease in expression of 'protamine', a marker of differentiated germ cells. In conclusion, these results suggest that metformin affects the testicular energy content and the proliferative ability of Sertoli and germ cells.

Characterization of chicken Sertoli cells in vitro.

In the testis, Sertoli cells play a key physiological role in that they support, nourish, and protect germ cells. Because of the importance of Sertoli cells, several laboratories have established a culture system of Sertoli cells. These cultures have been well developed in mammalian species, but to our knowledge no purified avian Sertoli cells culture has been described. The aim of this study was to isolate avian Sertoli cells and to investigate their function using a chicken model in an in vitro test system. Immature chicken Sertoli cells in culture present morphology similar to that of mammalian cells and conserve expression of the specific Sertoli marker, anti-Müllerian hormone. Furthermore, in contrast to mammals, they express the 3ß-hydroxysteroid dehydrogenase enzyme. Stimulation of Sertoli cells with ovine follicle-stimulating hormone rapidly activates the 3 main downstream signaling pathways of the follicle-stimulating hormone receptor: cyclic( )adenosine monophosphate/protein kinase A, phosphatidylinositol 3-kinase/Akt, and mitogen-activated protein kinase pathways. In vitro, Sertoli cells are able to secrete lactate and inhibin and have conserved the phagocytosis property. Finally, avian Sertoli cells present 3 interesting characteristics: they actively proliferate in vitro, can be passaged several times, and are suitable for freezing in nitrogen. A direct consequence of these properties is to use this cell culture test system as an alternative method to bird reprotoxicity studies.

A reappraisal of the factors involved in in vitro initiation of the acrosome reaction in chicken spermatozoa.

Chicken spermatozoa may remain in the female oviduct for a prolonged period before induction of the acrosome reaction on contact with the inner perivitelline layer (IPVL). By contrast, the acrosome reaction may be induced very rapidly in vitro in the presence of IPVL and Ca(2+). In the present study, we examined the extent to which the chicken acrosome reaction can be induced in media of various compositions in the presence or absence of IPVL and/or Ca(2+) and other factors known to be efficient in mammals. We also compared the efficacy of perivitelline layer (PL) taken at various states of oocyte maturation in initiating the reaction. The acrosome reaction was induced in less than 5 min in the presence of Ca(2+) and IPVL. Incubation of spermatozoa in different saline media (Beltsville poultry semen extender (BPSE); Dulbecco's modified eagle medium; NaCl-TES buffer) without IPVL showed a significant induction of acrosome reaction in BPSE supplemented with 5 mM Ca(2+) and in the three media after supplementation with Ca(2+) and Ca(2+) ionophore A23187. By contrast, the acrosome reaction was never induced without Ca(2+). BSA, NaHCO(3), and progesterone did not stimulate the acrosome reaction. Ca(2+) plus PL taken at various physiological states (follicle IPVL, ovulated IPVL, oviposited IPVL, and/or outer perivitelline layer) strongly stimulated the acrosome reaction, the latest states being the most efficient. Although PL induced the acrosome reaction in the presence of extracellular Ca(2+), it was not possible to induce hyperactivation in chicken spermatozoa. Taken together, these results emphasize the central role of Ca(2+) in the in vitro initiation of the acrosome reaction in chickens and show specific features of this induction in birds.

Effects of exposing chicken eggs to a cell phone in "call" position over the entire incubation period.

The aim of the present study was to assess the effects of exposing fertile chicken eggs to a cell phone repeatedly calling a ten-digit number at 3-min intervals over the entire period of incubation. A pre-experiment was performed first to adjust incubation conditions in an experimental chamber devoid of metallic content and without automatic turning until the overall performance of hatchability was reproducible in the absence of the cell phone. The experimental period consisted of a series of 4 incubations referred to as "replicates". For each replicate, one batch of 60 eggs was exposed to the immediate environment (

Duration of fertility and hatchability of the common duck (Anas platyrhynchos) in pure- or crossbreeding with Muscovy drakes (Cairina moschata).

A total of 540 common duck dams were used for a comparison of duration of fertility and hatchability between eggs issued from common dams inseminated with sperm (175 x 10(6) dose(-1)) from either common (pure-breeding or PB) or Muscovy (crossbreeding or CB) drakes. Artificial inseminations (AI) were performed at 3 periods of the reproductive season (27-35, 39-43 and 49-56 weeks) with 2 alternate inseminations/period at 3-week intervals (one with semen from common and the other from Muscovy). Fertility was estimated from egg candling while early embryo mortality (EEM), medium embryo mortality (MEM) and late embryo mortality (LEM) was estimated on Days 0-6 (PB+CB), Days 7-25 (PB) or Day 28 (CB) of incubation, and after, respectively. Overall fertility from Days 2-12 after AI was 61.1% in PB and 42.8% in CB. The maximum duration of fertility (time interval between AI and last fertile egg) was 8.1 days in PB versus 6.4 days in CB (p<0.05). The age of the dam influenced this interval, particularly in PB, with a longer duration at 40 weeks compared to 50 (p<0.05). On average, EEM represented 2.5% of fertile eggs while MEM accounted for 5% of surviving embryos on Day 6 and LEM, for 11.5% of hatched eggs. MEM was significantly higher in CB (6.3%) compared to PB (3.9%; p<0.05). Overall, an increase in EEM and MEM was observed in both types of eggs at and after 50 weeks of age. An increase in EEM (regardless of dam's age) and in MEM (only in the oldest females) was observed with sperm storage duration. Sex ratio at hatching (49.2% males in PB vs. 53.0% in CB) was particularly unbalanced on the first fertile day (54.7% and 57.1%, respectively).

Morphological and histochemical characterization of the seminiferous epithelial and Leydig cells of the turkey.

Unlike mammals, there is little fundamental information about spermatogenesis in birds. This study was undertaken to clarify the morphology, histochemistry, and lectin affinity of the seminiferous epithelial cells and Leydig cells in pre-pubertal (8- to 15-week old) and adult (40- to 44-week old) domestic turkeys. In adult turkeys, three types of spermatogonia were defined based on their chromatin distribution and nuclear morphology: the dark type A (A(d)); the pale type A (A(p)); and the type B. The A(d) is the least numerous and least conspicuous and consequently difficult to locate. Based on its spatial distribution and overall morphology, type A(d) spermatogonia were postulated to be the spermatogonia stem cells in the turkey. Antibodies to c-kit were localized to spermatogonia in the pre-pubertal and to a lesser extent in adult males. Peanut agglutinin (PNA) was specific for spermatocytes in the pre-pubertal males and spermatogonia and early spermatocytes in adult males. Wheat-germ agglutinin (WGA) highlighted Sertoli cells in both age groups. Bandeiraea simplicifolia I, soybean agglutinin, and winged-pea agglutinin staining were limited to the wall of the seminiferous tubule and some extra-tubular cell types. Concanavalin A staining was diffuse and not cell-specific and, therefore, could not be used to selectively identify a particular cell type. It was concluded that WGA and PNA could aid in identifying specific cell types in the seminiferous epithelium of testis from pre-pubertal and mature turkeys. Only Leydig cells were alkaline phosphatase reactive in the mature turkey testes. The information from this study is being used to adapt techniques for the isolation and partial purification developed for mammalian spermatogonia to avian spermatogonia and other specific cell types in the testes.

Timing associated with oviductal sperm storage and release after artificial insemination in domestic hens.

Female birds store sperm in sperm storage tubules (SSTs) in the uterovaginal junction of their reproductive tract for days or weeks (depending on species) before fertilization. Sperm are transported from the SSTs to the infundibulum where fertilization occurs immediately after ovulation of each ovum. The timing of sperm release from the SSTs relative to ovulation is unknown for any bird. Here, we show that, after artificial insemination of domestic fowl Gallus domesticus, sperm are not accepted into any region of the oviduct before sexual maturity. Once hens reach maturity, there is a temporal shift in the distribution of sperm throughout the oviduct. Sperm are first accepted into and accumulate in the SSTs 6 to 8 days before ovulation but are at this point significantly less numerous in the infundibulum. From 1 to 6 days before ovulation, approximately 10-fold more sperm (235 × 10(3) sperm) populate the infundibulum than at 6 to 8 days before ovulation (26 × 10(3) sperm; P < 0.001). Our results suggest that the mechanisms underlying sperm acceptance and release in the oviduct are under fine temporal control, most likely mediated by female hormones.

Fatty acid composition, glutathione peroxidase and superoxide dismutase activity and total antioxidant activity of avian semen.

This work demonstrates that spermatozoa from five avian species (chicken, turkey, guinea fowl, duck and goose) are all characterised by high proportions of polyunsaturated fatty acids, from 46 (turkey) to 55% (duck) of total. For each of the species, the most abundant fatty acids were arachidonic (20:4n-6) and docosatetraenoic (22:4n-6) acids, representing between 22 (turkey) and 40% (chicken) of total. Significant activities of the major isozymes of superoxide dismutase and glutathione peroxidase, which protect against the peroxidation associated with high degree of fatty acid unsaturation, were found in spermatozoa from all species. The seminal plasma also had these activities and showed additional mechanisms for protecting spermatozoa from peroxidation. In general terms, these lipid and enzyme proteins were similar between the five avian species and different from those reported for mammalian sperm.

Migration of spermatozoa in the oviduct of hens following intravaginal, intramagnal and intraabdominal insemination.

When hens were inseminated intravaginally with 200 million spermatozoa, the largest number of sperm cells reaching the infundibulum was observed 2 d after insemination (41.64 x 10(3) per female), even though a few sperm (0.23 x 10(3) per female) had already been detected within the first hour following insemination. After 2 d, the number of spermatozoa rapidly decreased and only 4.09 x 10(3) sperm per female were present in the infundibulum on Days 14 and 21, respectively. However, when the same dose of spermatozoa was inseminated intramagnally, a large number of spermatozoa (8.01 x 10(3) per female) was found in the infundibulum within 4 h after insemination. A parallel study showed that extensive migration of spermatozoa towards the abodminal cavity had already occurred.

Comparison of assessment of fowl sperm viability by eosin-nigrosin and dual fluorescence (SYBR-14/PI).

The kinetics of fowl sperm viability/mortality following short-term and long-term in vitro storage were studied using 2 different staining methods: eosin/nigrosin (observed under light microscopy) and SYBR-14/PI (dual fluorescence). Based on data obtained at 0, 30 min and at 2, 4 and 24 h (T0, T30, T2, T4, and T24) after in vitro storage (4 degrees C, agitated) of fresh or frozen-thawed semen, the dual association SYBR-14/PI was more effective than eosin/nigrosin (P < 0.05) staining for the detection of sperm viability/mortality at early stages (30 min) in nonfrozen ejaculates stored above 0 degree C. In cryopreserved preparations, the 2 techniques were comparable for assessing viable spermatozoa immediately after thawing, but higher percentages (P < 0.05) of nonviable spermatozoa were detected by the SYBR-14/PI procedure for up to 4 h of in vitro storage post thawing (4 degrees C, agitated). Finally, comparable results were observed between the 2 techniques 24 h after beginning in vitro storage post thawing. It is concluded that the dual association SYBR-14/PI procedure is more effective (or, at least, more rapid) than eosin/nigrosin staining for the assessment of sperm viability/mortality in both fresh and cryopreserved samples of fowl semen. However, in the latter case, the thawing stage needs to be followed by a period of in vitro storage lasting at least 4 h to allow for easier discrimination between viable and nonviable populations of spermatozoa.

Phospholipid fatty acid composition, vitamin E content and susceptibility to lipid peroxidation of duck spermatozoa.

Recent studies on chicken semen have suggested that the lipid and fatty acid composition of spermatozoa may be important determinants of fertility. Phospholipid fatty acid composition, vitamin E content and in vitro susceptibility to lipid peroxidation of duck spermatozoa were investigated using GC-MS and HPLC based methods. The total phospholipid fraction of duck spermatozoa was characterized by high proportions of the n-6 polyunsaturated fatty acids arachidonic (20:4n-6), docosatetraenoic (22:4n-6) and docosapentaenoic (22:5n-6) acids but a substantial proportion of the n-3 fatty acid docosahexaenoic (22:6n-3) acid was also present. Palmitic (16:0) and stearic (18:0) fatty acids were the major saturates in sperm phospholipids. Among the phospholipid classes, phosphatidylserine (PS) had the highest degree of unsaturation due to very high proportions of 22:6n-3, 22:5n-6, 22:4n-6 and 20:4n-6, comprising together more than 75% of total fatty acids in this fraction. Phosphatidylethanolamine (PE) also contained high proportions of these four C(20-22) polyunsaturates, which together formed 60% of total fatty acids in this phospholipid. Spermatozoa and seminal plasma of duck semen were characterized by unexpectedly low content of vitamin E, being more than 4-fold lower than in chicken semen. In duck semen the major proportion of the vitamin E (>70%) was located in the spermatozoa. The very high proportion of 22:6n-3 in PS and PE fractions of duck sperm lipids and the comparatively low levels of vitamin E could predispose semen to lipid peroxidation. Nevertheless the in vitro susceptibilities to Fe2+-stimulated lipid peroxidation of duck and chicken spermatozoa were very similar. The results of the study suggest that increased superoxide dismutase and glutathione peroxidase activity and increased antioxidant activity of seminal plasma may compensate for the low levels of vitamin E to help protect the membranes of duck spermatozoa, which exhibit a high degree of unsaturation from oxidative stress.

Comparison of bacteriological qualities of various egg yolk sources and the in vitro and in vivo fertilizing potential of bovine semen frozen in egg yolk or lecithin based diluents.

The addition of components of animal origin (egg yolk, milk) to most commercial diluents used to freeze bull semen represents a potential risk of contamination of the doses with bacteria or mycoplasma. A series of quantitative and qualitative analyses were performed to detect microbiological contamination observed in Biociphos plus (a new lecithin-glycerol based freezing salt buffer), in an egg yolk diluent (Triladyl) or in an egg yolk + milk-based (Laiciphos) diluent of bull semen. The 2 diluents containing animal products showed moderate (10 to 60 CFU/mL) contamination (17/17 samples) with bacteria or mycoplasma, or both, while no contamination was observed in the 6 examined batches of Biociphos plus. Biociphos plus was also compared with another commercial diluent (Laiciphos) for use in freezing bull semen intended for in vitro and/or in vivo fertilization. No difference (P > 0.05) could be detected between the 2 diluents for in vitro fertility rates (percentage of cleaved zygotes: 85.7% and 88.0%, respectively, for Laiciphos and Biociphos plus). Similarly, 2 series of comparisons conducted in dairy cows artificially inseminated with semen frozen in either Biociphos plus or Laiciphos showed no difference in fertilizing capacity (tested at 60 to 90 d; P > 0.05) irrespective of the age of the bulls (Trial 1, bulls aged 14 to 15 m.o.; Trial 2, bulls aged 2 to 5 yr, field trials). It is concluded that, in addition to maintaining the fertilizing capacity of bull semen at levels comparable to those observed with standard freezing diluent, Biociphos plus also prevents microbiological contamination by bacteria or mycoplasma, both of which are generally present in the various commercially available sources of egg yolk.

Sex ratios in mule duck embryos at various stages of incubation.

Mule duck hatcheries have long reported varying degrees of unbalance in the sex ratio, with a preponderance of male mules at hatching. The aim of the present study was to assess the distributions of sex ratios at various stages of development in embryos originating from intra- and intergeneric crosses between parental lineages (Muscovy male x Muscovy female, Pekin male x Pekin female, Muscovy male x Pekin female or Mule, and Pekin male x Muscovy female or Hinny). In Experiment I, embryo sexing was performed on Days 1 and 5 of incubation (by multiplex PCR) and at hatching (by vent observation). The sex ratio was not significantly modified during the early stages of embryo development whatever the genetic origin (P>0.05, Days 1 and Day 5) but our results in mule and hinny ducklings confirmed the preponderance of males among normally hatched ducklings originating from the intergeneric lineage (58.9 and 55.4% males in mules and hinnies, respectively; P<0.05 in both cases). Sex ratio (vent sexing) in second grade (cull) ducklings revealed that 68% of these ducklings were females (P<0.05). In Experiment II, the distribution of sex ratio was also performed in mule duck eggs from 6 batches (400,000 eggs/batch) first examined for fertility (candling) on Day 18 of incubation. These results indicate that the percentage of males present in the population of normally hatched ducklings increases when fertility decreases. In addition, this experiment also revealed that 83.7-90.5% of viable male mule embryos develop up to hatching, compared to only 43.0-51.0% of female mule embryos. Given that a deviation in sex ratio during the first stages of incubation is unlikely (Experiment I), it is concluded that the skewed sex ratio of mule ducks at hatching is primarily due to increased late mortality in female mule embryos occurring between egg transfer and hatching. This mortality originated, at least in part, from the intergeneric origin of female mules, and was marked to a greater or lesser extent depending on the initial success of fertilization in a given batch, a possible indication that the initial quality of gametes may selectively exert its influence at the later stages of embryo development.

Sperm storage and transport following natural mating and artificial insemination.

Recent observations in turkey and chicken hens show that sperm storage in both species is a highly inefficient process. After artificial insemination (AI), less than 1% of spermatozoa inseminated are selected for transport to and enter the sperm storage tubules (SST). It has been shown that the sperm selection process is orchestrated within the vagina and not at the level of the SST. At least two mechanisms are involved in the selection of spermatozoa fit for sperm storage, one being mechanical (motility) and the other biochemical in nature (sperm-vaginal mucosa interactions). Furthermore, it was also observed that the sperm storage efficiency in the chicken is dependent upon the logarithm of the number of spermatozoa inseminated. From a practical standpoint, inseminations performed frequently with a moderate number of spermatozoa should be more efficient than inseminations performed with higher doses at longer intervals. Maximal filling of the SST of hens in egg production requires only 1 day for the chicken and 2 days for the turkey. By contrast, the release of sperm from the SST is about seven times faster in the chicken than the turkey hen. The efficiency of oviducal sperm storage is related to a number of factors including age of the hen, stage of the ovulatory cycle when inseminated, and, in the turkey, if the hen was inseminated before or after the onset of egg production. Two different categories should be considered among factors that affect sperm survival in vivo. 1) Factors affecting sperm storage.(ABSTRACT TRUNCATED AT 250 WORDS)

Age-related variations in seminiferous tubule dimensions and germinal and Sertoli cell numbers in guinea-fowl raised under a 14L:10D photoperiod.

Histological studies of testicular development in guinea-fowl (Numida meleagris), raised under a 14L:10D photoperiod from 1 to 70 weeks of age, revealed: rapid increases in the relative volume, diameter, and length of the seminiferous tubules from 8 to 20 weeks but no significant changes thereafter; the appearance at 12 weeks of both mature Sertoli cells and round spermatids, characteristic of puberty; and biphasic increases in the numbers of Sertoli and germinal cells. The numbers of Sertoli cells, Type I spermatocytes, and round spermatids increased rapidly between 8 and 20 weeks; thereafter the numbers of Sertoli cells and Type I spermatocytes increased slowly but significantly, whereas the number of round spermatids was static. This indicated that age-related changes in meiotic yields could occur in adult guinea-fowl maintained under a 14L:10D photoperiod.

Influence of spermatozoa numbers and insemination frequency on fertility in dwarf broiler breeder hens.

The effects of hen age (28 to 31 vs. 49 to 52 weeks of age), sperm concentration (dose used for artificial insemination), and frequency of insemination on fertility and embryonic survival of dwarf broiler breeder hens were examined. Hens in Groups 1 and 2 were inseminated weekly with single doses of either 250 million (Group 1) or 125 million (Group 2) sperm during the 4 weeks of each period. Hens in Groups 3 and 4 were inseminated every other week with duplicate doses on 2 consecutive days, with 250 million sperm/dose in Group 3 and 125 million/dose in Group 4. Hens in Groups 5 and 6 were inseminated weekly with either 250 million (Group 5) or 125 million (Group 6) sperm dose, except the 1st week of each period when they received duplicate doses as in Groups 3 and 4. In Groups 1 and 2, insemination with weekly single doses of semen (250 or 125 million sperm) had no significant effect on fertility of young or old hens. Percent fertility during the 2nd week after artificial insemination was lower in Group 4 than in Group 3 (73.0 vs. 82.9 in young hens and 70.4 vs. 80.7 in old hens). There were no significant differences in fertility between semen doses or age periods in Groups 5 and 6. In these two groups, overall fertility ranged from 94.3 to 95.9%. Complementary studies on individual fertility and embryonic survival showed the beneficial effects of duplicate followed by single inseminations of moderate doses (125 million sperm) practiced at weekly intervals in old hens. This method should be of practical application in commercial practice.

Effects of frequency of semen collection on quantitative and qualitative characteristics of semen in turkey breeder males.

The effects of various frequencies of semen collection on several quantitative and qualitative semen characteristics were investigated in adult turkey breeder males (30 to 40 wk of age). In Experiment 1, a total of 35 males were first trained for semen collection (twice a week for 2 consecutive wk), and then divided into five groups (seven males each), each group being collected either once every 2 wk, once every week, twice every week, three times every week (each for 4 wk) or five to seven times per week (each for 2 wk). Volume, sperm concentration, and sperm number per ejaculate were determined for each ejaculate. No significant differences between groups were observed for sperm concentration (P > 0.05), but males collected once every 2 wk, once per week, or twice per week had larger volumes than males collected at higher frequencies (P < 0.05). Thus there were significant differences for sperm number per ejaculate between groups (P < 0.05). Also, daily semen output (DSO) was markedly increased in males collected at the highest frequencies (e.g., DSO = 0.62 x 10(9) and 1.93 x 10(9) in males collected once and five times per week). Finally, in euthanatized birds (36 wk) no differences between groups were observed for body weight (25.8 +/- 1.7 kg), testicular weight (51.5 +/- 2.2 g), or total number of elongated spermatids per male (14.0 +/- 0.8 x 10(9)). In Experiment 2, 35 males were distributed into groups and collected under the same conditions as in Experiment 1. Besides quantitative analyses of ejaculates (volume, sperm concentration, and sperm per ejaculate), sperm viability between groups was also tested using the Sybr14/PI fluorescence test. Our results demonstrated: 1) a favorable effect of high semen collection frequencies on sperm viability and, 2) a marked decline in sperm viability during the first 2 d following a 2-d resting period in males collected five times a week. We concluded that turkey males express their optimal reproductive capacity more efficiently when semen collection is undertaken at a high rather than a low frequency.

The reliability and efficiency of various methods for estimating spermatozoa concentration.

A study was conducted of the reliability and the efficiency of four methods to estimate concentration of spermatozoa in chicken semen. The methods used were hemocytometer, Coulter counter, optical density, and spermatocrit. Twenty-four samples of pooled semen (5 males per sample) were used in this experiment. Sperm concentration estimates were determined on each of three subsamples: pure semen, semen diluted 1:1, and semen diluted 1:3. The average time to prepare and evaluate 6 replications of each subsample with the hemocytometer, Coulter counter, optical density, and spermatocrit methods was 9.0, 2.6, 2.3, and 4.4 min, respectively. Correlation coefficients ranged from .78 to .93 between the hemocytometer and either optical density or Coulter counter in both pure and diluted 1:1 and 1:3 samples. However, no significant correlation was observed between the hemocytometer and spermatocrit in the 1:3 dilution. The reliability expressed as coefficient of variation for each technique was: hemocytometer 17.9%, Coulter counter 1.57%, optical density 2.24%, and spermatocrit 9.95%. It is concluded from these results that the optical density and Coulter counter methods are more reliable and more efficient (less time consuming) than either hemocytometer or spermatocrit methods in estimating semen concentrations in chickens.

Testis development and daily sperm output in guineas submitted to progressively increasing daily photoperiods at different ages.

Four hundred and eighty guineas were raised under short days (7L:17D) from 3 weeks of age, then subjected to increasing light at 8, 16, 20, or 24 weeks of age. After receiving 7 additional hours of light (+ 1 hr per week) for each of 7 consecutive weeks, each group was then maintained on long days (14L:10D) until 70 weeks of age. No significant differences were observed between photoschedules for growth rate or adult body weight; however, the age at which the daylengths were increased greatly influenced the development of the testes and daily sperm output (DSO). The earlier the age birds were submitted to increasing light, the sooner the rapid phase of testis growth occurred and the lower adult testicular weight. Results were similar in the mean DSO expressed as a function of the age or photoschedule. Male guineas preconditioned by short days and submitted to increasing daylength from 20 weeks of age appeared to reach sperm production sufficiently early to inseminate contemporary females as they started to lay. Sperm production was high enough to ensure insemination of 6 to 12 females per male instead of the usual 3 to 4 under the present management conditions in the industry.

Maternal body weight and feed allowance of breeders affect performance of dwarf broiler breeders and tibial ossification of their progeny.

Four hundred and eight dwarf broiler breeder hens were raised collectively in a floor pen to 21 wk of age. At this age they were classified into four groups with reference to their individual BW as heavy (1.95 +/- .1 kg), medium (1.80 +/- .1 kg), light (1.69 +/- .1 kg), and ultralight (1.57 +/- .1 kg). All groups were individually caged at 23 wk of age. During the reproductive period, each group was divided into three subgroups fed on liberal, intermediate, or severe feed restriction (reaching up to 135, 125, and 115 g of daily feed allowance at 29 wk of age, respectively). Intergroup differences in BW were maintained throughout the experiment (21 to 61 wk) but tended to decrease with age. Hen-day egg production was depressed by the lower feed allowance. Fertility and hatchability were impaired when hens received the largest quantities of food. Hen size influenced female breeder performance only slightly. Shell quality and albumen quality were affected by the level of feed consumption. Egg weights as well as BW of the progeny at hatching were enhanced by increased maternal BW and feed allowance. This positive maternal effect was still present at 40 days of age. Despite better overall BW performances of the male versus female broilers, the abdominal fat pad of female broilers was heavier than that of males and tended to increase with breeder size and breeder feed allowance. Accordingly, tibial breaking strength and percentage ash of the progeny at hatching were markedly improved in proportion to the breeders' BW and to their feed allowance. The effect of breeder size on broiler tibial quality was maintained up to 40 days of age but the effect of breeder feed intake tended to disappear with increasing age of the broilers. Tibial strength and mineralization were higher in male than in female broilers at 40 days of age. Dyschondroplasia was higher in broilers hatched from heavier breeder hens, but was not influenced by breeder feed intake. The incidence of varus and valgus in progeny was similar whatever the breeders' treatment. It is concluded that performance of dwarf breeders in a given flock depends mainly upon breeder feed allowance but that broiler performance and, especially, tibial ossification of broilers is greatly influenced by maternal size and, to a lesser extent, by maternal feed intake.