Transfer of mlt mutations into polyomavirus intronless genomes by intramolecular recombination in bacteria

We describe a modification of the procedure of Weber and Weissmann [Nucl. Acids Res. 11 (1983) 5661-5669] for the formation of hybrid genes by in vivo recombination to introduce two separate mutations into the same gene. The mutants of interest are inserted as head-to-tail tandems in a bacterial plasmid in such a way that the 5'-proximal mutation is located upstream from the mutant with the more distal mutation. Propagation of the plasmid in a rec+ strain of Escherichia coli allows recombination between homologous sequences in the insert. DNA with the size expected for the recombinant plasmid is isolated by agarose gel electrophoresis, cloned in a recA strain, and characterized by restriction endonuclease mapping. Using this procedure, we have transferred the deletion from polyomavirus mutant dl-8 into other mutant genomes lacking the intervening sequences for either middle T or large T.     

Polyoma middle T antigen requires cooperation from another gene to express the malignant phenotype in vivo.

The oncogenic potential of polyomavirus in newborn hamsters can be expressed by a recombinant encoding only the middle T protein. However, polyoma middle T requires the cooperation from small T to induce tumors in newborn rats. Similar complementary functions such as cocarcinogens or tumor promotors can be exerted by the simian virus 40 T antigens as well as by one or several products of the early region 1A of adenovirus 2.     

Elements of the polyomavirus replication origin required for homologous recombination mediated by large T antigen.

We introduced various elements of the polyomavirus origin of DNA replication into the genome of rat cells, and we analyzed their capacity to elicit rearrangements within the integrated sequences when exposed to large T antigen. The cis-acting sequences required for homologous recombination were those that make up a functional replication origin.     

Effects of birth on energy metabolism in the rat kidney.

The oxygen-consumption rates and the activities of fumarase and beta-hydroxyacyl-CoA dehydrogenase were compared in mitochondria isolated from fetal- and neonatal-rat kidney. Whole-organ ATP, phosphocreatine and creatine contents were determined in parallel. Kidney mitochondrial respiratory rates in the presence of succinate, glutamate/malate and palmitoyl-L-carnitine increased between 21 days post coitum and 1 day post partum, together with activities of oxidative enzymes. However, this postnatal maturation of oxidative metabolism was not yet initiated in mitochondria isolated from kidney 1 h post partum. An increase in ATP and phosphocreatine was observed immediately after delivery; newborn-rat kidney ATP content then remained high, whereas phosphocreatine reserves decreased considerably between 6 h and 1 day post partum. It is concluded that the increase in high-energy phosphate compounds observed at birth is not initially related to an activation of oxidative phosphorylation, and probably involves a transient stimulation of anaerobic glycolysis, while a progressive mitochondrial maturation takes place in the rat kidney during the first day of newborn life.     

The Leishmania donovani chaperone cyclophilin 40 is essential for intracellular infection independent of its stage‐specific phosphorylation status

During its life cycle, the protozoan pathogen Leishmania donovani is exposed to contrasting environments inside insect vector and vertebrate host, to which the parasite must adapt for extra‐ and intracellular survival. Combining null mutant analysis with phosphorylation site‐specific mutagenesis and functional complementation we genetically tested the requirement of the L. donovani chaperone cyclophilin 40 (LdCyP40) for infection. Targeted replacement of LdCyP40 had no effect on parasite viability, axenic amastigote differentiation, and resistance to various forms of environmental stress in culture, suggesting important functional redundancy to other parasite chaperones. However, ultrastructural analyses and video microscopy of cyp40?/? promastigotes uncovered important defects in cell shape, organization of the subpellicular tubulin network and motility at stationary growth phase. More importantly, cyp40?/? parasites were unable to establish intracellular infection in murine macrophages and were eliminated during the first 24 h post infection. Surprisingly, cyp40?/? infectivity was restored in complemented parasites expressing a CyP40 mutant of the unique S274 phosphorylation site. Together our data reveal non‐redundant CyP40 functions in parasite cytoskeletal remodelling relevant for the development of infectious parasites in vitro independent of its phosphorylation status, and provide a framework for the genetic analysis of Leishmania‐specific phosphorylation sites and their role in regulating parasite protein function.     

Proteomic Analysis of Intact Flagella of Procyclic Trypanosoma brucei Cells Identifies Novel Flagellar Proteins with Unique Sub-localization and Dynamics

Cilia and flagella are complex organelles made of hundreds of proteins of highly variable structures and functions. Here we report the purification of intact flagella from the procyclic stage of Trypanosoma brucei using mechanical shearing. Structural preservation was confirmed by transmission electron microscopy that showed that flagella still contained typical elements such as the membrane, the axoneme, the paraflagellar rod, and the intraflagellar transport particles. It also revealed that flagella severed below the basal body, and were not contaminated by other cytoskeletal structures such as the flagellar pocket collar or the adhesion zone filament. Mass spectrometry analysis identified a total of 751 proteins with high confidence, including 88% of known flagellar components. Comparison with the cell debris fraction revealed that more than half of the flagellum markers were enriched in flagella and this enrichment criterion was taken into account to identify 212 proteins not previously reported to be associated to flagella. Nine of these were experimentally validated including a 14-3-3 protein not yet reported to be associated to flagella and eight novel proteins termed FLAM (FLAgellar Member). Remarkably, they localized to five different subdomains of the flagellum. For example, FLAM6 is restricted to the proximal half of the axoneme, no matter its length. In contrast, FLAM8 is progressively accumulating at the distal tip of growing flagella and half of it still needs to be added after cell division. A combination of RNA interference and Fluorescence Recovery After Photobleaching approaches demonstrated very different dynamics from one protein to the other, but also according to the stage of construction and the age of the flagellum. Structural proteins are added to the distal tip of the elongating flagellum and exhibit slow turnover whereas membrane proteins such as the arginine kinase show rapid turnover without a detectible polarity.Cilia and flagella are prominent organelles of many eukaryotic cells. The names “cilia” and “flagella” are often related to historical reasons but they correspond to the same entity: a cylindrical organelle surrounded by a membrane and composed of an axoneme, a set of nine doublet microtubules originating from the basal body. Motile cilia usually contain a central pair of single microtubules and various substructures involved in the generation or the control of flagellar or ciliary beating, such as dynein arms, radial spokes, or central pair projections. This structural organization is remarkably well conserved across evolution, being encountered from protists to mammals (1). The conservation is also found at the molecular level as observed by comparative genomics between species with or without cilia and flagella (2, 3). Nevertheless, proteomic analysis revealed that in addition to the common core, many components unique to each group of eukaryotes are also present (4–8).The cilium represents a separate compartment from the cell body and does not contain any ribosomes or vesicles of any kind. The base of cilia and flagella contains projections that link each microtubule triplet of the basal body to the flagellum membrane (9). This region has been proposed to act as a barrier restricting entry of cytoplasmic proteins and ensuring retention of flagellum matrix elements (10). The transition zone is found in-between this area and the axoneme and contains several complexes of proteins (many of whom are mutated in the case of ciliopathies, genetic diseases affecting cilia function and/or formation) that contribute to the definition of the ciliary compartment (11, 12). Recent data showed that dextrans of low molecular weight are free to diffuse in the ciliary compartment as well as in the nucleus, whereas molecules of higher size (30 kDa or above) could not access these organelles. This led to the finding that a structure equivalent to the nucleopore complex is localized at the basal body area and could control access to the ciliary compartment (13). Finally, a septin barrier appears to be present close to the basis of the cilium and could control the trafficking of specific ciliary membrane proteins (14). The existence of a specific compartment comprising a large number of skeletal, matrix, and membrane proteins raises the issue of its internal organization. Key questions include the distribution of proteins, the mechanisms involved in specific distribution and the turnover during the life of the organelle.We selected to address these basic phenomena in the protist Trypanosoma brucei, well known as the etiological agent of sleeping sickness in Africa, but that is also an amenable model for cilia studies (15). It possesses a single flagellum that contains a typical 9 + 2 axoneme emerging from a depression of the cell surface called the flagellar pocket. This structure can be related to the ciliary pocket found at the base of different types of cilia in mammalian cells (16, 17). The axoneme is flanked by a lattice-like structure called the paraflagellar rod (PFR)¹ that is present as soon as the flagellum emerges from the pocket and runs to its distal end (18). The PFR contains at least 30 different proteins (19) and has been proposed to contribute to cell motility because its ablation results in cell paralysis in T. brucei (20) and in the related parasite Leishmania mexicana (21). The flagellum is attached to the cell body for most of its length, with the PFR lying close to the cell body side where a specific cytoskeletal structure termed the flagellum attachment zone (FAZ) is found (22). It is made of a unique filament composed of trypanosome-specific proteins (23, 24) and of four specialized microtubules flanked by the smooth endoplasmic reticulum (25). The flagellum plays key cellular functions as it drives cell motility (4, 26, 27), controls cell morphogenesis (28) and is responsible for parasite attachment during invasion of the salivary glands in the tsetse fly (29). Moreover, it could perform sensory functions and contribute to detection of the environment during the parasite life cycle (30). Recent data revealed the essential role of flagellum beating during fly invasion (31) but surprisingly reduction of forward motility did not affect infectivity in a mouse model (32).Purification of intact flagella from trypanosomes is a challenging task because of the adhesion to the cell body. Detergent and high-salt treatment have been used to efficiently purify the skeletal fraction of the flagellum that contains the axoneme, the PFR, and the basal body but that also includes the kinetoplast (mitochondrial genome), the FAZ, and the flagellar pocket collar (4, 33, 34). However, membrane and matrix components are totally lost during this procedure. For example, none of the intraflagellar transport (IFT) proteins that normally traffic in the flagellum matrix along peripheral microtubules (35) could be detected in samples purified by this procedure (4). We therefore decided to purify intact flagella by using a mutant strain called FLA1^RNAi where expression of an mRNA encoding a protein essential for flagellum attachment to the cell body (36) can be conditionally knocked-down by RNAi (37). FLA1^RNAi cells exhibit detached flagella from the main cell body, with the exception of the anchoring point at the basal body (37). By mechanical shearing, we found out that flagella could be severed from the cell body while preserving their membrane and their matrix elements. After purification, flagellar fractions were exhaustively characterized at the level of light and electron microscopy and their content was determined by mass spectrometry that confirmed the presence of the majority of known flagellar markers and revealed novel flagellar components. Three previously characterized proteins (the arginine kinase and two 14-3-3 proteins) and 10 hypothetical proteins were investigated in detail. Out of these 13 candidate proteins, 10 turned out to be associated to the flagellum whereas the others could not be detected experimentally. The novel ones were termed FLAM, for Flagellum Members. Remarkably, these proteins showed very specific location patterns within the flagellum including the membrane, the distal tip of the axoneme or the first proximal half of the axoneme, and displayed unexpected variations in their turnover rate. Overall, we revealed the existence of multiple subdomains within the flagellum with very specific dynamics, further demonstrating the highly sophisticated organization of the organelle.     

Optimization, production, and partial characterization of an alkalophilic amylase produced by sponge associated marine bacterium Halobacterium salinarum MMD047

An endosymbiont Halobacterium salinarum MMD047, which could produce high yields of amylase, was isolated from marine sponge Fasciospongia cavernosa, collected from the peninsular coast of India. Maximum production of enzyme was obtained in minimal medium supplemented with 1% sucrose. The enzyme was found to be produced constitutively even in the absence of starch. The optimum temperature and pH for the enzyme production was 40°C and 8.0, respectively. The enzyme exhibited maximum activity in pH range of 6∼10 with an optimum pH of 9.0. The enzyme was stable at 40°C and the enzyme activity decreased dramatically above 50°C. Based on the present findings, the enzyme was characterized as relatively heat sensitive and alkalophilic amylase which can be developed for extensive industrial applications.