Defective retrograde transport impairs autophagic clearance in Alzheimer disease neurons

Macroautophagy/autophagy plays a key role in cellular quality control by eliminating protein aggregates and damaged organelles, which is essential for the maintenance of neuronal homeostasis. Defective autophagy has been implicated in the pathogenesis of Alzheimer disease (AD). In AD brains, autophagic vacuoles (AVs) accumulate massively within dystrophic neurites. This raises a fundamental question as to whether impaired autophagic clearance contributes to AD-associated autophagic stress. We recently revealed that AD neurons display defective retrograde transport and accumulation of amphisomes predominantly in axons and presynaptic terminals. Amyloid β (Aβ) oligomers are enriched in axons and interact with dynein motors. This interaction interferes with the coupling of the dynein motor with its adaptor SNAPIN. Such deficits disrupt dynein-driven retrograde transport of amphisomes, thus trapping them in distal axons and impairing their degradation in the soma. Therefore, our study provides new mechanistic insights into AD-linked autophagic pathology, and builds a foundation for developing potential AD therapeutic strategies by rescuing retrograde transport of amphisomes.     

Cellular Internalization of Exosomes Occurs Through Phagocytosis

Exosomes play important roles in many physiological and pathological processes. However, the exosome–cell interaction mode and the intracellular trafficking pathway of exosomes in their recipient cells remain unclear. Here, we report that exosomes derived from K562 or MT4 cells are internalized more efficiently by phagocytes than by non‐phagocytic cells. Most exosomes were observed attached to the plasma membrane of non‐phagocytic cells, while in phagocytic cells these exosomes were found to enter via phagocytosis. Specifically, they moved to phagosomes together with phagocytic polystyrene carboxylate‐modified latex beads (biospheres) and were further sorted into phagolysosomes. Moreover, exosome internalization was dependent on the actin cytoskeleton and phosphatidylinositol 3‐kinase, and could be inhibited by the knockdown of dynamin2 or overexpression of a dominant‐negative form of dynamin2. Further, antibody pretreatment assays demonstrated that tim4 but not tim1 was involved in exosomes uptake. We also found that exosomes did not enter the internalization pathway involving caveolae, macropinocytosis and clathrin‐coated vesicles. Our observation that the cellular uptake of exosomes occurs through phagocytosis has important implications for exosome–cell interactions and the exosome intracellular trafficking pathway.     

Late dormant rapeseed oil treatment against black cherry aphid and cherry fruit moth in sweet cherries

Abstract:  Black cherry aphid [ Myzus cerasi (Fabricius)] and cherry fruit moth [ Argyresthia pruniella (Clerck)] are the main insect pests on sweet cherries in Norway. In this study, application of rapeseed oil alone and rapeseed oil mixed with pesticides were tested as a control method against overwintering eggs of both black cherry aphid and cherry fruit moth. Results showed that rapeseed oil applied at the late dormant stage significantly reduced damage by black cherry aphid. Efficiency of oil mixed with pesticides was higher, but only significant in three of seven trials. The efficiency of rapeseed oil against cherry fruit moth was low compared with what was achieved for black cherry aphid, but within the range that has been reported for other botanical pesticides. As for the black cherry aphid, adding pesticides to oil decreased damage by the cherry fruit moth. Timing of treatment and effect of temperature were discussed.     

Interpretation of the last‐glacial vegetation of eastern‐central Europe using modern analogues from southern Siberia

Aim Interpretation of fossil pollen assemblages may benefit greatly from comparisons with modern palynological and vegetation analogues. To interpret the full‐ and late‐glacial vegetation in eastern‐central Europe we compared fossil pollen assemblages from this region with modern pollen assemblages from various vegetation types in southern Siberia, which presumably include the closest modern analogues of the last‐glacial vegetation of central Europe. Location Czech and Slovak Republics (fossil pollen assemblages); Western Sayan Mountains, southern Siberia (modern pollen assemblages). Methods Eighty‐eight modern pollen spectra were sampled in 14 vegetation types of Siberian forest, tundra and steppe, and compared with the last‐glacial pollen spectra from seven central European localities using principal components analysis. Results Both full‐ and late‐glacial pollen spectra from the valleys of the Western Carpathians (altitudes 350–610 m) are similar to modern pollen spectra from southern Siberian taiga, hemiboreal forest and dwarf‐birch tundra. The full‐glacial and early late‐glacial pollen spectra from lowland river valleys in the Bohemian Massif (altitudes 185–190 m) also indicate the presence of patches of hemiboreal forest or taiga. Other late‐glacial pollen spectra from the Bohemian Massif suggest an open landscape with steppe or tundra or a mosaic of both, possibly with small patches of hemiboreal forest. Main conclusions Our results are consistent with the hypothesis that during the full glacial and late glacial, the mountain valleys of the north‐western Carpathians supported taiga or hemiboreal forest dominated by Larix, Pinus cembra, Pinus sylvestris and Picea, along with some steppic or tundra formations. Forests tended to be increasingly open or patchy towards the west (Moravian lowlands), gradually passing into the generally treeless landscape of Bohemia, with possible woodland patches in locally favourable sites.     

Potato Expressed Sequence Tag Generation and Analysis using Standard and Unique cDNA Libraries

To help develop an understanding of the genes that govern the developmental characteristics of the potato (Solanum tuberosum), as well as the genes associated with responses to specified pathogens and storage conditions, The Canadian Potato Genome Project (CPGP) carried out 5′ end sequencing of regular, normalized and full-length cDNA libraries of the Shepody potato cultivar, generating over 66,600 expressed sequence tags (ESTs). Libraries sequenced represented tuber developmental stages, pathogen-challenged tubers, as well as leaf, floral developmental stages, suspension cultured cells and roots. All libraries analysed to date have contributed unique sequences, with the normalized libraries high on the list. In addition, a low molecular weight library has enhanced the 3′ ends of our sequence assemblies. Using the combined assembly dataset, unique tuber developmental, cold storage and pathogen-challenged sequences have been identified. A comparison of the ESTs specific to the pathogen-challenged tuber and foliar libraries revealed minimal overlap between these libraries. Mixed assemblies using over 189,000 potato EST sequences from CPGP and The Institute for Genomics Research (TIGR) has revealed common sequences, as well as CPGP- and TIGR-unique sequences. Electronic Supplementary Material Electronic Supplementary material is available for this article at and accessible for authorised users.     

Mannose 6-phosphate receptors, Niemann-Pick C2 protein, and lysosomal cholesterol accumulation

Niemann-Pick disease type C (NPC), caused by mutations in the NPC1 gene or the NPC2 gene, is characterized by the accumulation of unesterified cholesterol and other lipids in endo/lysosomal compartments. NPC2 is a small, soluble, lysosomal protein that is targeted to this compartment via a mannose 6-phosphate-inhibitable pathway. To obtain insight into the roles of mannose 6-phosphate receptors (MPRs) in NPC2 targeting, we here examine the trafficking and function of NPC2 in fibroblast lines deficient in one or both of the two MPRs, MPR46 and MPR300. We demonstrate that either MPR alone is sufficient to transport NPC2 to the endo/lysosomal compartment, although MPR300 seems to be more efficient than MPR46. In the absence of both MPRs, NPC2 is secreted into the culture medium, and only a small amount of intracellular NPC2 can be detected, mainly in the endoplasmic reticulum. This leads to massive accumulation of unesterified cholesterol in the endo/lysosomal compartment of the MPR46/300-deficient fibroblasts, a phenotype similar to that of the NPC patient fibroblasts. In addition, we observed an upregulation of NPC1 protein and mRNA in the MPR-double-deficient cells. Taken together, our results suggest that the lysosomal targeting of NPC2 is strictly dependent on MPRs in fibroblasts.     

On the biogenesis of myelin membranes: Sorting, trafficking and cell polarity

In the central nervous system, a multilayered membrane layer known as the myelin sheath enwraps axons, and is required for optimal saltatory signal conductance. The sheath develops from membrane processes that extend from the plasma membrane of oligodendrocytes and displays a unique lipid and protein composition. Myelin biogenesis is carefully regulated, and multiple transport pathways involving a variety of endosomal compartments are involved. Here we briefly summarize how the major myelin proteins proteolipid protein and myelin basic protein reach the sheath, and highlight potential mechanisms involved, including the role of myelin specific lipids and cell polarity related transport pathways.     

NSF independent fusion of Salmonella-containing late phagosomes with early endosomes

Initial characterizations of live-Salmonella-containing early (LSEP) and late phagosomes (LSLP) in macrophages show that both phagosomes retain Rab5 and EEA1. In addition, LSEP specifically contain transferrin receptor whereas LSLP possess relatively more rabaptin-5. In contrast to LSLP, late-Salmonella-containing vacuoles in epithelial cells show significantly reduced levels of Rab5 and EEA1. Subsequent results demonstrate that both phagosomes efficiently fuse with early endosomes (EE). In contrast to LSEP, fusion between LSLP and EE is insensitive to ATPγS treatment. Furthermore, LSLP fuses with EE in absence of NEM-sensitive fusion factor (NSF) as well as in the presence of NSF:D1EQ mutant demonstrating that LSLP fusion with EE is NSF independent.