Reproductive Competition in Colonies of the Ant Leptothorax gredleri

Colonies of the ant, Leptothorax (s. str.) gredleri may contain several inseminated female reproductives of which typically only one is laying eggs. Observations suggest that “functional monogyny” is caused by aggressive interactions among nestmate queens. Only the most dominant queen reproduces. Subordinate queens either leave the colony to found their own nests solitarily or by budding, or stay in the nest without reproducing, but may eventually replace the dominant queen. The interrelations of life history of L. gredleri, population structure and habitat characteristics are examined.     

A new anaerobic,sporing, acetate-oxidizing,sulfate-reducing bacterium,Desulfotomaculum (emend.) acetoxidans

Archives of Microbiology - A new strictly anaerobic, polarly flagellated, sporing, acetate-oxidizing, sulfate-reducing bacterium was isolated from anaerobic fresh or sea water mud samples. The...     

Die Rezeptoren an den ersten Antennen vonLeptestheria dahalacensis Rüppel (Crustacea,Conchostraca)

Zusammenfassung Bei dem ConchostracenLeptestheria dahalacensis kommen auf den ersten Antennen etwa 600 gleich aussehende Sinneshaare vor, die in Gruppen von jeweils 25–30 zusammengefaßt sind. Diese Sinneshaare sind in zwei Teile gegliedert, die durch das lichtmikroskopisch gut sichtbare Basalstück (basal bead) voneinander getrennt sind. Dieses bildet die Basis des Haares, dessen Wand im wesentlichen aus Epicuticula besteht. Apikal wird das Haar durch das Endkügelchen (terminal pellet) abgeschlossen. Das Basalstück wird von der untersten Lage der Epicuticula gebildet. Die 4–10 Receptorcilien, die jeweils einzeln ebensovielen Dendriten aufsitzen, ziehen aus dem inneren Teil des Rezeptors, der von insgesamt 5 Hüllzellen umgeben wird, durch das Basalstück, in dem sie stark eingeengt werden und verzweigen sich dann im äußeren Teil des Rezeptors. Sie ziehen bis zum Endkügelchen, in das sie durch einen Porus, den man als Häutungsporus ansprechen kann, eintreten. In der Häutungsvorbereitung wird der Haarbalg von der Hüllzelle 5, das Basalstück von der Hüllzelle 4, der Haarschaft dagegen von der Hüllzelle 3 gebildet. Dabei spaltet sich die Hüllzelle 3 ringspaltförmig auf, so daß in diesem Spalt der neuangelegte Haarschaft handschuhfingerförmig eingestülpt liegt. Die Hüllzelle 2 formt die Spitze des neuen Haares, während die Dendritenscheide von der Hüllzelle 1 abgegeben wird.

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The receptors on the first antennae ofLeptestheria dahalacensis Rüppel (Crustacea, Conchostraca)

Summary On the antennulae ofLeptestheria dahalacensis (Conchostraca) nearly 600 sensory setae of one type are found. They are gathered in groups of 25–30. The single sensory seta is divided into two parts by the basal bead which is easily visible in the light microscope. The basal bead is the socket of the seta, whose wall is mainly built up by the epicuticle. The terminal pellet closes the tip of the seta. The basal bead is derived from the innermost layer of the epicuticle. 4–10 dendrites each with one receptorcilium innervate the receptor. The receptorcilia stretch through the interior part of the receptor and the basal bead into the exterior part, where they branch. They enter the terminal pellet in a porus, which seems to be a moulting porus. The interior part of the receptor is surrounded by 5 sheath cells. During the premoult it becomes obvious, that the socket of the seta is built by the sheath cell 5, the basal bead by the sheath cell 4 and the shaft by the sheath cell 3. For this the sheath cell 3 is divided into two parts. Between this two parts the newly formed cuticle is invaginated. The sheath cell 2 formes the tip and the sheath cell 1 the cuticular sheath of the new bristle.

     

Surfactant protein D increases phagocytosis and aggregation of pollen-allergen starch granules

Recent studies have shown that surfactant components, in particular the collectins surfactant protein (SP)-A and -D, modulate the phagocytosis of various pathogens by alveolar macrophages. This interaction might be important not only for the elimination of pathogens but also for the elimination of inhaled allergens and might explain anti-inflammatory effects of SP-A and SP-D in allergic airway inflammation. We investigated the effect of surfactant components on the phagocytosis of allergen-containing pollen starch granules (PSG) by alveolar macrophages. PSG were isolated from Dactylis glomerata or Phleum pratense, two common grass pollen allergens, and incubated with either rat or human alveolar macrophages in the presence of recombinant human SP-A, SP-A purified from patients suffering from alveolar proteinosis, a recombinant fragment of human SP-D, dodecameric recombinant rat SP-D, or the commercially available surfactant preparations Curosurf and Alveofact. Dodecameric rat recombinant SP-D enhanced binding and phagocytosis of the PSG by alveolar macrophages, whereas the recombinant fragment of human SP-D, SP-A, or the surfactant lipid preparations had no effect. In addition, recombinant rat SP-D bound to the surface of the PSG and induced aggregation. Binding, aggregation, and enhancement of phagocytosis by recombinant rat SP-D was completely blocked by EDTA and inhibited by d-maltose and to a lesser extent by d-galactose, indicating the involvement of the carbohydrate recognition domain of SP-D in these functions. The modulation of allergen phagocytosis by SP-D might play an important role in allergen clearance from the lung and thereby modulate the allergic inflammation of asthma.     

Inhibition of IL-6, TNF-alpha, and cyclooxygenase-2 protein expression by prostaglandin E2-induced IL-10 in bone marrow-derived dendritic cells

Several endogenously produced mediators, including cytokines such as IL-6, IL-10, and TNF-alpha and prostanoids such as prostaglandin E(2) (PGE(2)), regulate dendritic cell (DC) function and contribute to immune homeostasis. In this study, we report that exogenous PGE(2) enhances the production of IL-10 from bone marrow-derived DC (BM-DC). IL-6, but not TNF-alpha, release is enhanced by PGE(2) in the presence of anti-IL-10, suggesting that endogenous IL-10 masks PGE(2)-induced IL-6. Furthermore, both exogenous IL-10 and PGE(2) inhibit LPS-induced IL-6 and TNF-alpha, whereas selective inhibition of cyclooxygenase-2 (COX-2) or addition of anti-IL-10 causes the reverse effects. Exogenous IL-10, but not IL-6, dose-dependently suppresses COX-2 protein expression and PGE(2) production, and TNF-alpha does not reverse this effect. In contrast, anti-IL-10 up-regulates prostanoid production by LPS-stimulated BM-DC. Taken together, our results show that in response to PGE(2), BM-DC produce IL-10, which in turn down-regulates their own production of IL-6-, TNF-alpha-, and COX-2-derived prostanoids, and plays crucial roles in determining the BM-DC pro-inflammatory phenotype.     

Canine antibody response to Phlebotomus perniciosus bites negatively correlates with the risk of Leishmania infantum transmission

Background

Phlebotomine sand flies are blood-sucking insects that can transmit Leishmania parasites. Hosts bitten by sand flies develop an immune response against sand fly salivary antigens. Specific anti-saliva IgG indicate the exposure to the vector and may also help to estimate the risk of Leishmania spp. transmission. In this study, we examined the canine antibody response against the saliva of Phlebotomus perniciosus, the main vector of Leishmania infantum in the Mediterranean Basin, and characterized salivary antigens of this sand fly species.

Methodology/Principal Findings

Sera of dogs bitten by P. perniciosus under experimental conditions and dogs naturally exposed to sand flies in a L. infantum focus were tested by ELISA for the presence of anti-P. perniciosus antibodies. Antibody levels positively correlated with the number of blood-fed P. perniciosus females. In naturally exposed dogs the increase of specific IgG, IgG1 and IgG2 was observed during sand fly season. Importantly, Leishmania-positive dogs revealed significantly lower anti-P. perniciosus IgG2 compared to Leishmania-negative ones. Major P. perniciosus antigens were identified by western blot and mass spectrometry as yellow proteins, apyrases and antigen 5-related proteins.

Conclusions

Results suggest that monitoring canine antibody response to sand fly saliva in endemic foci could estimate the risk of L. infantum transmission. It may also help to control canine leishmaniasis by evaluating the effectiveness of anti-vector campaigns. Data from the field study where dogs from the Italian focus of L. infantum were naturally exposed to P. perniciosus bites indicates that the levels of anti-P. perniciosus saliva IgG2 negatively correlate with the risk of Leishmania transmission. Thus, specific IgG2 response is suggested as a risk marker of L. infantum transmission for dogs.     

Expression and Processing of a Small Nucleolar RNA from the Epstein-Barr Virus Genome

Small nucleolar RNAs (snoRNAs) are localized within the nucleolus, a sub-nuclear compartment, in which they guide ribosomal or spliceosomal RNA modifications, respectively. Up until now, snoRNAs have only been identified in eukaryal and archaeal genomes, but are notably absent in bacteria. By screening B lymphocytes for expression of non-coding RNAs (ncRNAs) induced by the Epstein-Barr virus (EBV), we here report, for the first time, the identification of a snoRNA gene within a viral genome, designated as v-snoRNA1. This genetic element displays all hallmark sequence motifs of a canonical C/D box snoRNA, namely C/C′- as well as D/D′-boxes. The nucleolar localization of v-snoRNA1 was verified by in situ hybridisation of EBV-infected cells. We also confirmed binding of the three canonical snoRNA proteins, fibrillarin, Nop56 and Nop58, to v-snoRNA1. The C-box motif of v-snoRNA1 was shown to be crucial for the stability of the viral snoRNA; its selective deletion in the viral genome led to a complete down-regulation of v-snoRNA1 expression levels within EBV-infected B cells. We further provide evidence that v-snoRNA1 might serve as a miRNA-like precursor, which is processed into 24 nt sized RNA species, designated as v-snoRNA1^24pp. A potential target site of v-snoRNA1^24pp was identified within the 3′-UTR of BALF5 mRNA which encodes the viral DNA polymerase. V-snoRNA1 was found to be expressed in all investigated EBV-positive cell lines, including lymphoblastoid cell lines (LCL). Interestingly, induction of the lytic cycle markedly up-regulated expression levels of v-snoRNA1 up to 30-fold. By a computational approach, we identified a v-snoRNA1 homolog in the rhesus lymphocryptovirus genome. This evolutionary conservation suggests an important role of v-snoRNA1 during γ-herpesvirus infection.