ABSTRACT
Novel immunofluorescence resonance energy transfer (immuno-FRET) assays for both Bacillus cereus spores and Escherichia coli O157:H7 are reported. Both assays involve the use of dual (QSY-7 and Oregon Green 514-antibody)-labeled spores or vegetative bacteria, such that Oregon Green 514-labeled antibodies are quenched by proximal QSY-7 molecules that are covalently bound to the dual (Oregon Green 514 and QSY-7)-labeled cells. Upon introduction of unlabeled bacteria or spores, in the respective assays, an increase in fluorescence is observed in proportion to the numbers of unlabeled cells. This is due to migration of Oregon Green 514-labeled antibody from the dual-labeled cells to the unlabeled target cells as verified by fluorescence microscopy. Optimization of the QSY-7 surface density led to a B. cereus spore detection sensitivity of approximately 1.0 x 10(5) to 2.5 x 10(5) spores per milliliter and 3.5 x 10(5) cells per milliliter for E. coli using a conventional cuvette-based spectrofluorometer.
Subject(s)
Bacillus cereus/isolation & purification , Escherichia coli O157/isolation & purification , Fluorescent Antibody Technique , Spores, Bacterial/isolation & purification , Energy Transfer , Fluoresceins/metabolism , Fluorescent Dyes/metabolism , Food Microbiology , Microscopy, Fluorescence , Molecular Structure , Reproducibility of Results , Sensitivity and Specificity , Spectrometry, FluorescenceABSTRACT
Axoplasmic organelles in the giant axon of the squid have been shown to move on both actin filaments and microtubules and to switch between actin filaments and microtubules during fast axonal transport. The objectives of this investigation were to identify the specific classes of axoplasmic organelles that move on actin filaments and the myosin motors involved. We developed a procedure to isolate endoplasmic reticulum (ER) from extruded axoplasm and to reconstitute its movement in vitro. The isolated ER vesicles moved on exogenous actin filaments adsorbed to coverslips in an ATP-dependent manner without the addition of soluble factors. Therefore myosin was tightly bound and not extracted during isolation. These vesicles were identified as smooth ER by use of an antibody to an ER-resident protein, ERcalcistorin/protein disulfide isomerase (EcaSt/PDI). Furthermore, an antibody to squid myosin V was used in immunogold EM studies to show that myosin V localized to these vesicles. The antibody was generated to a squid brain myosin (p196) that was classified as myosin V based on comparisons of amino acid sequences of tryptic peptides of this myosin with those of other known members of the myosin V family. Dual labeling with the squid myosin V antibody and a kinesin heavy chain antibody showed that the two motors colocalized on the same vesicles. Finally, antibody inhibition experiments were performed with two myosin V-specific antibodies to show that myosin V motor activity is required for transport of vesicles on actin filaments in axoplasm. One antibody was made to a peptide in the globular tail domain and the other to the globular head fragment of myosin V. Both antibodies inhibited vesicle transport on actin filaments by greater than 90% compared to controls. These studies provide the first direct evidence that ER vesicles are transported on actin filaments by myosin V. These data confirm the role of actin filaments in fast axonal transport and provide support for the dual filament model of vesicle transport.
Subject(s)
Actin Cytoskeleton/physiology , Actins/physiology , Egg Proteins , Endoplasmic Reticulum, Smooth/metabolism , Molecular Motor Proteins , Myosins/physiology , Neurons/metabolism , Protein Isoforms/physiology , Adenosine Triphosphate/metabolism , Amino Acid Sequence , Animals , Antibodies, Monoclonal/immunology , Biological Transport, Active , Biomarkers , Calcium-Binding Proteins/immunology , Decapodiformes , Models, Biological , Molecular Sequence Data , Nerve Tissue Proteins/immunology , Nerve Tissue Proteins/isolation & purification , Nerve Tissue Proteins/physiology , Optic Lobe, Nonmammalian/chemistry , Sequence Alignment , Sequence Homology, Amino Acid , Species SpecificityABSTRACT
Fast axonal transport is characterized by the bidirectional, microtubule-based movement of membranous organelles. Cytoplasmic dynein is necessary but not sufficient for retrograde transport directed from the synapse to the cell body. Dynactin is a heteromultimeric protein complex, enriched in neurons, that binds to both microtubules and cytoplasmic dynein. To determine whether dynactin is required for retrograde axonal transport, we examined the effects of anti-dynactin antibodies on organelle transport in extruded axoplasm. Treatment of axoplasm with antibodies to the p150(Glued) subunit of dynactin resulted in a significant decrease in the velocity of microtubule-based organelle transport, with many organelles bound along microtubules. We examined the molecular mechanism of the observed inhibition of motility, and we demonstrated that antibodies to p150(Glued) disrupted the binding of cytoplasmic dynein to dynactin and also inhibited the association of cytoplasmic dynein with organelles. In contrast, the anti-p150(Glued) antibodies had no effect on the binding of dynactin to microtubules nor on cytoplasmic dynein-driven microtubule gliding. These results indicate that the interaction between cytoplasmic dynein and the dynactin complex is required for the axonal transport of membrane-bound vesicles and support the hypothesis that dynactin may function as a link between the organelle, the microtubule, and cytoplasmic dynein during vesicle transport.
Subject(s)
Axonal Transport/physiology , Axons/metabolism , Cytoplasm/metabolism , Dyneins/metabolism , Microtubule-Associated Proteins/metabolism , Animals , Antibodies/pharmacology , Biological Transport/drug effects , Cell-Free System , Decapodiformes , Dynactin Complex , Microtubule-Associated Proteins/immunology , Microtubules/drug effects , Microtubules/ultrastructure , Organelles/physiology , Protein BindingABSTRACT
The mature form of cathepsin D (Cat D), purified to homogeneity from postmortem human brain or mouse brain, behaved as a 42-kDa protein in its native state but revealed additional proteolytic processing under denaturing conditions. Human brain Cat D was composed of a 30-32 kDa heavy chain and a protein doublet consisting of 14 and 15 kDa light chains. Mouse Cat D, which closely resembled the human enzyme in amino acid composition, existed mainly as the uncleaved 42-kDa protein, but up to 40% existed as a complex of 30-32 kDa and 12-14 kDa chains. The 3:1 ratio of light to heavy (30-32 kDa) chains suggested processing of some 30-kDa chains. Cleavage of the 42-kDa chain could not be induced autolytically. Human brain Cat D had a 2-3-fold higher specific activity than the mouse enzyme but shared other properties, including similar biphasic pH optima (peaks at pH 3.30 and 4.2), Km values for methemoglobin and inhibitor profiles. Human Cat D displayed the same polypeptide chain composition when purified from brains differing in postmortem interval (3-28 h). Fresh SH-SY5Y human neuroblastoma cells analyzed on Western blots with anti-Cat D antibodies also displayed only cleaved forms of mature Cat D. Furthermore, brain Cat D isolated from mice stored after death for 5, 15 or 30 h at 25 degrees C contained the same molar ratios of cleaved and uncleaved enzyme found in fresh mouse brain . Cat D activity was stable in human brains with postmortem intervals up to 27 h and stored frozen for up to 3 years. Similarly, total Cat D activity was essentially unchanged in brains of mice subjected to stimulated postmortem conditions for 0.5-4.2 h, although 20% of the total soluble brain protein became insoluble during this postmortem interval. These results demonstrate a remarkable postmortem stability of Cat D and strongly suggest that limited proteolytic cleavage of mature brain Cat D is an in vivo event, the extent of which varies markedly in different species.
Subject(s)
Aging/metabolism , Brain/metabolism , Cathepsin D/chemistry , Cathepsin D/metabolism , Peptide Hydrolases/metabolism , Aged , Animals , Drug Stability , Humans , Immunoblotting , Mice , Mice, Inbred C57BL , Neuroblastoma/metabolism , Neuroblastoma/pathology , Postmortem Changes , Time Factors , Tumor Cells, CulturedABSTRACT
Differentiation of skeletal muscle and the formation of the neuromuscular junction are regulated by steroid hormones. The effects of androgens on ion channel proteins central to neuromuscular signalling have been investigated in differentiating mouse muscle C2 cells and in C2 cells that stably overexpress the rat androgen receptor (AR) cDNA. Neither the expression nor function of ACh receptors was regulated by androgenic actions in these cells. However, voltage-dependent sodium (Na) current density was decreased by androgen treatment of C2 cells and was abolished, even in the absence of androgens, in C2 cells that overexpress the AR. The decrease in functional Na current was not accompanied by concomitant decreases in Na channel mRNA, suggesting that AR influence posttranscriptional processing of Na channels in differentiating C2 cells.
Subject(s)
Dihydrotestosterone/pharmacology , Muscles/physiology , Receptors, Androgen/physiology , Sodium Channels/physiology , Acetylcholine/pharmacology , Androgen Antagonists/pharmacology , Animals , Bungarotoxins/metabolism , Cell Differentiation , Cell Line , Flutamide/analogs & derivatives , Flutamide/pharmacology , Gene Expression , Metribolone/metabolism , Mice , Muscles/cytology , Muscles/metabolism , Rats , Receptors, Androgen/biosynthesis , Receptors, Androgen/drug effects , Receptors, Cholinergic/biosynthesis , Receptors, Cholinergic/drug effects , Receptors, Cholinergic/metabolism , Sodium Channels/drug effects , TransfectionABSTRACT
Glutamate, the major excitatory neurotransmitter in the mammalian central nervous system, is transported into bovine synaptic vesicles in a manner that is ATP dependent and requires a vesicular electrochemical proton gradient. We studied the electrical and chemical elements of this driving force and evaluated the effects of chloride on transport. Increasing concentrations of Cl- were found to increase the steady-state ATP-dependent vesicular pH gradient (delta pH) and were found to concomitantly decrease the vesicular membrane potential (delta psi). Low millimolar chloride concentrations, which cause 3-6-fold stimulation of vesicular glutamate uptake, caused small but measurable increases in delta pH and decreases in delta psi, when compared to control vesicles in the absence of chloride. Nigericin in potassium buffers was used to alter the relative proportions of delta pH and delta psi. Compared to controls, at all chloride concentrations tested, nigericin virtually abolished delta pH and increased the vesicle interior positive delta psi. Concomitantly, nigericin increased ATP-dependent glutamate uptake in 0-1 mM chloride but decreased glutamate uptake in 4 mM (45%), 20 mM (80%), and 140 mM (75%) Cl- (where delta pH in the absence of nigericin was large). These findings suggest that either delta psi, delta pH, or a combination can drive glutamate uptake, but to different degrees. In the presence of 4 mM Cl-, where uptake is optimal, both delta psi and delta pH contribute to the driving force for uptake. When the extravesicular pH was increased from 7.4 to 8.0, more Cl- was required to stimulate vesicular glutamate uptake. In the absence of Cl-, as extravesicular pH was lowered to 6.8, uptake was over 3-fold greater than it was at pH 7.4. As extravesicular pH was reduced from 8.0 toward 6.8, less Cl- was required for maximal stimulation. Decreasing the extravesicular pH from 8.0 to 6.8 in the absence of Cl- significantly increased glutamate uptake activity, even though proton-pumping ATPase activity actually decreased about 45% under identical conditions. In the absence of chloride, nigericin increased glutamate uptake at all the pH values tested except pH 8.0. Glutamate uptake at pH 6.8 in the presence of nigericin was over 6-fold greater than uptake at pH 7.4 in the absence of nigericin. We conclude from these experiments that optimal ATP-dependent glutamate uptake requires a large delta psi and a small delta pH.(ABSTRACT TRUNCATED AT 400 WORDS)
Subject(s)
Cerebral Cortex/metabolism , Glutamates/metabolism , Synaptic Vesicles/metabolism , Adenosine Triphosphate/metabolism , Animals , Biological Transport/drug effects , Cattle , Chlorides/pharmacology , Glutamic Acid , Hydrogen-Ion Concentration , Membrane Potentials , Methylamines/metabolism , Nigericin/pharmacology , Synaptic Vesicles/drug effects , Synaptic Vesicles/physiologyABSTRACT
The ATP-dependent uptake of glutamate into synaptic vesicles isolated form mammalian brains is well characterized. Glutamate uptake requires an electrochemical proton gradient, is specific for glutamate over other amino acids, and is stimulated by chloride. To determine whether these characteristics are fundamental to the vesicular uptake system, vesicles were isolated from the brain and central nervous ganglia of several vertebrate and invertebrate species, which included goldfish, frogs, turtles, pigeons, rats, Drosophila, and crayfish, and these vesicles were assayed for glutamate uptake activity. ATP-dependent glutamate was found in all of the vertebrate species tested, but was not detected in Drosophila or crayfish vesicles. The nature of the vesicular uptake of glutamate was similar among all the vertebrates: the specificity for glutamate remained high, transport was energized by a vacuolar (V)-type ATPase, 2-4 mM chloride stimulated uptake three- to sixfold, and Km for glutamate was between 0.5 and 2 mM. While these major characteristics of the uptake system remained conserved among the vertebrates tested, minor differences were seen in glutamate specificity, the steady-state level of glutamate obtained in the vesicles, and Vmax of the glutamate uptake systems. These results indicate that the synaptic vesicle glutamate uptake system is present throughout the vertebrate class, and that while minor changes in the transport system have occurred, its major functional characteristics, such as stimulation by chloride and strict substrate specificity, have been conserved for over 350-400 million years.
