Germline genomic structure of the B10.A mouseTcra-V2 gene subfamily

 The number of mouse Tcra-V gene segments varies from one individual to another and is estimated to be about 100. Southern blot analysis revealed that most of the Tcra-V are organized in clusters composed of copies of Tcra-V belonging to different subfamilies. We analyzed in detail a Tcra-V subfamily and looked for new Tcra-V in order to improve the knowledge of the mouse Tcra locus organization. A series of genomic clones derived from the B10.A mouse strain enclosing these clusters was used to determined the structure of all the Tcra-V2. We were able to identify ten Tcra-V2. This study showed that the Tcra-V2 can be organized into three structural subgroups. The distribution of the genes along the Tcra locus, plus their structural organization, indicates that successive duplications occurred during the processes of expansion and contraction of the Tcra-V gene subfamilies. Several Tcra-V2 are also identical, indicating recent duplications. The most divergent Tcra-V2 differ by 7.4% nucleotides, leading to 5.2% differences in amino acid contents. Received: 8 August 1995 / Revised: 24 April 1996     

Plasma HIV-2 RNA According to CD4 Count Strata among HIV-2-Infected Adults in the IeDEA West Africa Collaboration

Background

Plasma HIV-1 RNA monitoring is one of the standard tests for the management of HIV-1 infection. While HIV-1 RNA can be quantified using several commercial tests, no test has been commercialized for HIV-2 RNA quantification. We studied the relationship between plasma HIV-2 viral load (VL) and CD4 count in West African patients who were either receiving antiretroviral therapy (ART) or treatment-naïve.

Method

A cross sectional survey was conducted among HIV-2-infected individuals followed in three countries in West Africa from March to December 2012. All HIV-2 infected-patients who attended one of the participating clinics were proposed a plasma HIV-2 viral load measurement. HIV-2 RNA was quantified using the new ultrasensitive in-house real-time PCR assay with a detection threshold of 10 copies/ mL (cps/mL).

Results

A total of 351 HIV-2-infected individuals participated in this study, of whom 131 (37.3%) were treatment naïve and 220 (62.7%) had initiated ART. Among treatment-naïve patients, 60 (46.5%) had undetectable plasma HIV-2 viral load (<10 cps/mL), it was detectable between 10-100 cps/mL in 35.8%, between 100-1000 cps/mL in 11.7% and >1000 cps/mL in 6.0% of the patients. Most of the treatment-naïve patients (70.2%) had CD4-T cell count ≥500 cells/mm³ and 43 (46.7%) of these patients had a detectable VL (≥10 cps/mL). Among the 220 patients receiving ART, the median CD4-T cell count rose from 231 to 393 cells/mm³ (IQR [259-561]) after a median follow-up duration of 38 months and 145 (66.0%) patients had CD4-T cell count ≤ 500 cells/mm³ with a median viral load of 10 cps/mL (IQR [10-33]). Seventy five (34.0%) patients had CD4-T cell count ≥ 500 cells/mm³, among them 14 (18.7%) had a VL between 10-100 cps/mL and 2 (2.6%) had VL >100 cps/mL.

Conclusion

This study suggests that the combination of CD4-T cell count and ultrasensitive HIV-2 viral load quantification with a threshold of 10 cps/mL, could improve ART initiation among treatment naïve HIV-2-infected patients and the monitoring of ART response among patients receiving treatment.     

A New LxxxA Motif in the Transmembrane Helix3 of Maize Aquaporins Belonging to the Plasma Membrane Intrinsic Protein PIP2 Group Is Required for Their Trafficking to the Plasma Membrane

Aquaporins play important roles in maintaining plant water status under challenging environments. The regulation of aquaporin density in cell membranes is essential to control transcellular water flows. This work focuses on the maize (Zea mays) plasma membrane intrinsic protein (ZmPIP) aquaporin subfamily, which is divided into two sequence-related groups (ZmPIP1s and ZmPIP2s). When expressed alone in mesophyll protoplasts, ZmPIP2s are efficiently targeted to the plasma membrane, whereas ZmPIP1s are retained in the endoplasmic reticulum (ER). A protein domain-swapping approach was utilized to demonstrate that the transmembrane domain3 (TM3), together with the previously identified N-terminal ER export diacidic motif, account for the differential localization of these proteins. In addition to protoplasts, leaf epidermal cells transiently transformed by biolistic particle delivery were used to confirm and refine these results. By generating artificial proteins consisting of a single transmembrane domain, we demonstrated that the TM3 of ZmPIP1;2 or ZmPIP2;5 discriminates between ER and plasma membrane localization, respectively. More specifically, a new LxxxA motif in the TM3 of ZmPIP2;5, which is highly conserved in plant PIP2s, was shown to regulate its anterograde routing along the secretory pathway, particularly its export from the ER.Aquaporins are of major importance to plant physiology, being essential for the regulation of transcellular water movement during growth and development (Maurel et al., 2008; Gomes et al., 2009; Heinen et al., 2009; Prado and Maurel, 2013; Chaumont and Tyerman, 2014). Aquaporins are small membrane proteins consisting of six transmembrane (TM) domains connected by five loops (A–E), and N and C termini facing the cytosol (Fig. 1A). They assemble as homotetramers and/or heterotetramers in the membrane, with each monomer acting as an independent water channel (Murata et al., 2000; Fetter et al., 2004; Gomes et al., 2009). Aquaporins form a highly divergent protein family in plants (Chaumont et al., 2001; Johanson et al., 2001), and this work focuses on the maize (Zea mays) plasma membrane intrinsic protein (ZmPIP) family (Chaumont et al., 2001). The regulation of the subcellular localization of these proteins is a key process controlling their density in the plasma membrane (PM) and, hence, their physiological roles (Hachez et al., 2013).Open in a separate windowFigure 1.Swapping TM3 of ZmPIP2;5 with that of ZmPIP1;2 retains the protein in intracellular structures. A, Cartoons representing the chimeric proteins composed of ZmPIP2;5, in which each TM has been replaced by the corresponding TM from ZmPIP1;2. All proteins are drawn with the cytosolic domains facing down. ZmPIP2;5 and ZmPIP1;2 portions are shown in black and white, respectively. All chimeras were fused to the C terminus of mYFP, which is not displayed for clarity purposes. B, Confocal microscopy images of maize mesophyll protoplasts transiently coexpressing mYFP-tagged ZmPIP2;5-PIP1;2 TM chimeric proteins (green) and the ER marker mCFP:HDEL (cyan). FM4-64 was added as a PM marker (red). Arrowheads in image 13 indicate accumulation of the protein in punctate structures that are not labeled by mCFP:HDEL. The localization patterns of the proteins of interest are representative of a total of at least 22 cells from three independent experiments. C, Confocal microscopy images of a maize mesophyll protoplast transiently expressing mYFP:ZmPIP2;5-TM3_PIP1;2 (green) and ST:mCFP (magenta). Arrowheads indicate colocalization in Golgi stacks. The images are representative of a total of 17 cells from two independent experiments. Bar = 5 µm.PIP aquaporins cluster in two groups (PIP1s and PIP2s), which are highly conserved across species (Kammerloher et al., 1994; Chaumont et al., 2000, 2001; Johanson et al., 2001; Anderberg et al., 2012). We previously showed that the maize PIP1 and PIP2 isoforms exhibit different water channel activities when expressed in Xenopus laevis oocytes, with only PIP2s increasing the membrane water permeability coefficient (P_f; Chaumont et al., 2000). However, when ZmPIP1 and ZmPIP2 are coexpressed, the isoforms physically interact to modify their stability and trafficking to the oocyte membrane, and synergistically increase the oocyte P_f (Fetter et al., 2004). Similar synergistic interactions between PIP1s and PIP2s have been reported in numerous plant species (Temmei et al., 2005; Mahdieh et al., 2008; Vandeleur et al., 2009; Bellati et al., 2010; Ayadi et al., 2011; Horie et al., 2011; Yaneff et al., 2014).PIPs were originally thought to be exclusively localized in the PM and were named accordingly (Kammerloher et al., 1994). However, recent experiments have shown that not all PIPs are located to the PM under all conditions, and that regulation of PIP subcellular localization is a highly dynamic process involving protein interactions (Boursiac et al., 2005, 2008; Zelazny et al., 2007, 2009; Uehlein et al., 2008; Besserer et al., 2012; Luu et al., 2012). When expressed singly in maize leaf mesophyll protoplasts, fluorescently tagged ZmPIP1s and ZmPIP2s differ in their subcellular localization. ZmPIP1s are retained in the endoplasmic reticulum (ER), whereas ZmPIP2s are targeted to the PM (Zelazny et al., 2007). However, upon coexpression, ZmPIP1s are relocalized from the ER to the PM, where they perfectly colocalize with ZmPIP2s. This relocalization results from their physical interaction as demonstrated by Förster resonance energy transfer/fluorescence lifetime imaging microscopy and immunoprecipitation experiments (Zelazny et al., 2007). These results indicate that ZmPIP2s, but not ZmPIP1s, possess signals that allow them to be delivered to the PM, and that hetero-oligomerization is required for ZmPIP1 trafficking to the PM. Interestingly, a diacidic motif (DxE, Asp-any amino acid-Glu) located in the N terminus of ZmPIP2;4, ZmPIP2;5, and Arabidopsis (Arabidopsis thaliana) AtPIP2;1 was shown to be required to exit the ER (Zelazny et al., 2009; Sorieul et al., 2011). Diacidic motifs interact with Secretory protein24, which is thought to be the main cargo-selection protein of the Coat proteinII complex that mediates vesicle formation at ER export sites (Miller et al., 2003). However, not all PM-localized PIP2s contain a diacidic ER export signal (Zelazny et al., 2009). In addition, swapping the N-terminal region of ER-retained ZmPIP1;2 with that of PM-localized ZmPIP2;5, which contains the functional diacidic motif, is not sufficient to trigger ER export of the protein (Zelazny et al., 2009). This result suggests that other export signals might be present in PIP2s and/or ER retention signals might be present in PIP1s elsewhere than in the N terminus.To identify new signals regulating ZmPIP1 and ZmPIP2 protein trafficking along the secretory pathway, we used a protein domain swapping-based approach and identified the TM3 as an important region that discriminates between ER-retained ZmPIP1;2 and PM-localized ZmPIP2;5. Specific mutations in the TM3 region of ZmPIP2;5 allowed the identification of a new ZmPIP2-conserved LxxxA motif, which regulates its export from the ER.     

Etude histologique,histochimique et ultrastructurale de la pars intercerebralis chez Locusta migratoria L. (Orthoptere)

Summary A histological, histochemical and ultrastrucutral study of the pars intercerebralis (PI) has been made in Locusta migratoria. The acellular neural lamella is made up of an elastic tissue and collagen fibrils. The cells of the perilemma contain numerous lysosome structures and lipid granules.Three different types of neurosecretory cells (NSC A, B and C) have been distinguished in the PI associated with giant neurons.The cells termed A and B seem not to have an activity cycle during the two last larval instars. At the moment of sexual maturity the NSC A show an important accumulation of neurosecretory material and their number increases at the expense of the NSC B. The NSC A, which are characterized by a highly developped endoplasmic reticulum, contain numerous secretory granules which appear to be individualized in the Golgi complex in three different ways. The NSC B, with a reduced endoplasmic reticulum and an almost quiescent Golgi complex, contain abundant lysosome structures and more seldom some neurosecretory granules. In fact, the study of the fine structure shows different intermediate types, linking in a continuous way typical A cells and typical B cells. NSC A and NSC B might correspond to two opposed stages of secretory activity of one single cell type: the A cell representing the activity stage and the B cell the quiescent stage.NSC C show an accumulation of their neurosecretory products in relation to metamorphosis and sexual maturity. Ultrastructural evidence confirms their neurosecretory activity.A mode of regulating neurosecretion in NSC A and B by internal catabolism of the secretion and formation of lysosome like structures is discussed in the present paper.The giant neurons, which are surrounded by a glial envelope (trophospongium), contain several dense granules originated from Golgi complex.     

Molecular phylogeny of the paper wasp subgenus Polistes (Polistella) Ashmead, 1904 (Hymenoptera: Vespidae: Polistinae) from Vietnam

This study provides the first molecular phylogeny of the social wasp subgenus Polistella (Hymenoptera: Vespidae: Polistes) from Vietnam. Fragments of the mitochondrial COI and 16S rRNA genes were used to reconstruct the phylogenetic trees among 38 Polistes species plus two out-group species (Vespa soror du Buysson and Ropalidia fasciata (Fabricius)). Our results support the existence of several species-groups, including two that are congruent with the previous stigma and Stenopolistes groups defined on the basis of morphology. Moreover, we recovered a clade including the stigma group and the two species P. humilis and P. variabilis that was sister to all other species of Polistella. However, the results also challenged the definition of other groups of Polistella based on morphological data, as well as the definition of two species: P. brunus and P. affinis. This first study calls for further analyses including morphological characters to clarify the taxonomy and the classification of the group.     

Sex allocation in haplodiploids is mediated by egg size: evidence in the spider mite Tetranychus urticae Koch

Haplodiploid species display extraordinary sex ratios. However, a differential investment in male and female offspring might also be achieved by a differential provisioning of eggs, as observed in birds and lizards. We investigated this hypothesis in the haplodiploid spider mite Tetranychus urticae, which displays highly female-biased sex ratios. We show that egg size significantly determines not only larval size, juvenile survival and adult size, but also fertilization probability, as in marine invertebrates with external fertilization, so that female (fertilized) eggs are significantly larger than male (unfertilized) eggs. Moreover, females with on average larger eggs before fertilization produce a more female-biased sex ratio afterwards. Egg size thus mediates sex-specific egg provisioning, sex and offspring sex ratio. Finally, sex-specific egg provisioning has another major consequence: male eggs produced by mated mothers are smaller than male eggs produced by virgins, and this size difference persists in adults. Virgin females might thus have a (male) fitness advantage over mated females.