Predation risk of eggs and nestlings relative to nest‐site characteristics of the Bull‐headed Shrike Lanius bucephalus

Appropriate nest‐site selection is one of the most important ways to minimize loss of reproductive investment due to predation. We determined the environmental characteristics associated with nest predation during the incubation and nestling periods of arboreal nesting Bull‐headed Shrikes on the oceanic Minami‐Daito Island where the predator community has low species diversity and includes only three introduced mammals: Ship Rat Rattus rattus, Japanese Weasel Mustela itatsi and Feral Cat Felis catus. Egg predation declined with increasing grassland cover around nests, whereas nestling predation declined with increasing nest concealment and nest height. Our results suggest that effective nest‐site characteristics for avoiding nest predation differ during the incubation and nestling periods and are dependent on the predator species and their search strategies, at least in habitats with low predator species diversity.     

中国东北地区兴安落叶松林树干呼吸的研究

树干呼吸是森林碳平衡估计中的一个重要项目同时还能够显示树木的活力.对于如何准确估计森林树干呼吸释放CO2总量还存在争论.在本项研究中,2001～2002连续两年在一个33年生的兴安落叶松(Larix gmelini Rupr.)人工林内对树干呼吸进行了测定,同时测定了不同高度树干呼吸、呼吸的日变化、同龄落叶松林内不同个体的树干呼吸以及相关生长状态因子、水分因子和温度因子.结果显示:1)树干上部的呼吸速率在不同季节都高于下部呼吸速率,树干温度的差异能够一定程度上解释这种差异;2)树干呼吸有午间降低的现象,上午的测定结果树干温度与树干呼吸速率紧密相关,而下午则温度依赖性很小,土壤、空气、小枝木质部水势、叶片蒸腾速率和气孔导度都显示下午植物水分亏缺下午较上午严重,呼吸的这种上下午温度相关性的差异可能受这种水分亏缺的影响;3)在同龄林内,树木个体生长状态包括平均生长速率和树冠投影面积与树干呼吸速率有显著相关关系,而树干温度与之相关性很小.幂指数模型和S曲线模型能够产生较好的拟合效果;4)树干呼吸季节变化明显,7月份出现最大值,但同一月份的年间差异较大.自然指数模型能够较好地拟合温度与树干呼吸的季节变化规律.Q10值在2.22(2001年)和3.53(2002年)之间,与以往研究的结果相当.从以上结果可以看出,通过单一的Q10值估计森林树干呼吸总量会产生偏差,要想得到准确的估计,至少应该考虑生长状态的差异和水分状态的差异.     

Isolation of microsatellite loci in the freshwater goby,Rhinogobius sp. (Gobiidae)

The Rhinogobius species complex (Pisces: Gobiidae) includes great variation in colour, morphology and ecological form. In particular, R. sp. OR (Orange type) exhibits some of the greatest colour variation among the species complex, although the genetic relationships among the variations in this fish remain unclear. Thirteen microsatellite loci were identified from R. sp. OR, and all loci were polymorphic with two to 17 alleles per locus. Observed heterozygosity ranged from 0.1 to 0.9, while the expected heterozygosity ranged from 0.19 to 0.96. Multiplex polymerase chain reaction reaction (PCR) were optimized. All loci except Rhi‐5 conform to Hardy–Weinberg equilibrium (P > 0.05).     

Expression of Toxin Receptors on Cell Surfaces in Transdifferentiating Cultures of Neural Retina

It has often been asked which of the cell types found during the early stages of culturing embryonic chick neural retina can undergo transdifferentiation into lens in vitro. Since neuronal cell-surface toxin receptors are maintained in NR cultures for much longer than internal neuronal enzymes (e.g. choline acetyltransferase), and since the transdifferentiation process can be greatly accelerated by preparing reaggregates of neural retina cells after about 10 days of preculture as "monolayers", a direct test of this question became feasible. 7 or 9 day embryonic chick neural retina cells, precultured for 10–12 days as monolayers, were dissociated and reaggregated under continuous gyration. Reaggregates were maintained for 8 days in the presence of either tetanus toxin or FITC-conjugated α-bungarotoxin, to permit surface-bound toxins to become internalised via receptor turnover. The reaggregates were then dissociated, stained with rabbit antitoxin and FITC-conjugated anti-antibody in the case of tetanus toxin-labelled material, and restained with a rat or mouse antibody against chick δ crystallin followed by the appropriate rhodamine-conjugated anti-antibody. Although both FITC/toxin-labelled cells (putative neurones) and rhodamine/δ crystallin-labelled cells (transdifferentiated lens cells) were abundant, no examples of double-labelled cells were observed with 9 day starting material, and only a very few with 7 day starting material. We conclude that the vast majority of differentiated neuronal cells expressing surface receptors for these toxins do not transdifferentiate directly into lens cells.     

Involvement of 14-nm Filament-Forming Protein and Tubulin in Gametic Pronuclear Behavior during Conjugation in Tetrahymena

We have studied in detail the immunofluorescence localizations of Tetrahymena 14-nm filament-forming protein (49-kDa protein) in relation to tubulin in conjugating wild-type Tetrahymena thermophila (B strain) pairs and in pairs between B strain and star strains with defective micronuclei. The results suggest that germ nuclear behavior during conjugation may involve the following cytoskeletal structures: (1) during meiosis, microtubule structures are involved in micronuclear elongation and meiotic division; (2) at the postmeiotic stage, 49-kDa protein network structures that are formed independently of the existence of pronuclei are involved in the selection and the survival of one of four meiotic products; (3) during the third prezygotic division, gametic pronuclear transfer, and zygote formation, a cytoskeletal structure in which the 49-kDa protein colocalizes with microtubules and which is dependent on the existence of a normal gametic pronucleus is involved in gametic pronuclear behavior, and (4) during the postzygotic divisions, the microtubules are involved in nuclear behavior.     

Can Once Neuronally Differentiated Cells of Neural Retina Be Lentoidogenic in Cell Culture?*

Cells dissociated from neural retina of 3.5-day-old chick embryos transdifferentiated extensively into lens cells under the conditions of a cell culture for 3 to 4 weeks. In early satges of cell culture by about 10 days, cultures consisted of small round cells often with cytoplasmic processes(N-cells) and flattened epithelial cells (E-cells). Only N-cells were stained with a fluorescent dye Merocyanine 540. When cells harvested from early cultures were separated into two fractions by centrifugation in Percoll gradient, the specific activity of choline acetyltransferase was much higher in the fraction consisting mainly of N-cells than in other fraction mainly of E-cells. Continuous daily observations as well as cinematographic observations of living cultures indicate that lentoid bodies were often formed in the locations where clusters of N-cells had been found in early stages of culturing. The possibility of transdifferentiation of N-cell clusters into lentoid bodies is discussed.     

FURTHER STUDY RE-EXAMINING WHETHER LARVAL EPIDERMIS CAN OMIT THE SECRETION OF A PUPAL CUTICLE, USING THE SILKWORM, BOMBYX MORI

When larval tissue is exposed to a hormonal milieu lacking juvenile hormone, adult characters appear directly, omitting the pupal stage, in some insects but not in others, including Bombyx mori. An attempt was made to induce omission of pupal characters in this species by varying the stage of the larval epidermis to be tested. Pieces of larval integument taken from fourth- and fifth-instar larvae of various stages were transplanted to developing adults. Although the number of cuticle layers and the types of cuticle produced differed depending on the age of the donors, none of the pieces omitted secreting the pupal cuticle. It is concluded that the larval epidermis cannot omit secreting pupal cuticle, and that a transition of tissue competence may play an important part in the sequential appearance of larval, pupal, and adult characters.     

Vicariance and dispersal in the differentiation of vocalization in the Ryukyu Scops Owl Otus elegans

The distribution of species and species diversity can be affected by vicariance or dispersal. To understand their role in shaping species distribution and population structure these two processes must be estimated within and among populations. I analysed large‐scale variation in the call structure of the Ryukyu Scops Owl Otus elegans. This owl is distributed over a 1200‐km range, and only inhabits islands. Within this range, I studied this species across 22 continental islands of the Ryukyu Archipelago and two oceanic islands. The study aimed to assess whether there is variation in the acoustic structure of Owl hoot calls within islands, among major groups of islands and across a large area comprising a major biogeographical barrier (the Kerama Gap). The acoustic structure of calls was homogeneous within islands and among major island‐groups. Acoustic differentiation, however, increased over longer geographical distances of up to about 1200 km. The acoustic structure of hoots of the Ryukyu Scops Owl populations was clearly divided into two groups, north and south of the Kerama Gap. It is suggested that the Kerama Gap acted as a biogeographical barrier and contributed to the differentiation between the two major island‐groups. It is likely that this difference developed during the fragmentation of a widespread ancestral population by vicariant isolating events. There was also evidence of an effect of dispersal on vocal differentiation in subspecies inhabiting the two oceanic islands.