2,858 research outputs found
Thermal sensitivity and activation energy of intrinsic intestinal motility in small vertebrates
1. 1.|In vitro thermal sensitivity (t.s.) of mammalian small intestine is significantly greater than t.s. of the gut of ectothermic vertebrates. In vitro contraction frequency (c.f.) of endothermic gut is an order of magnitude greater than ectothermic gut at equivalent temperatures.2. 2.|Gut contraction t.s. is generally consistent within a given order of mammals and differs between orders. Differences in gut contraction t.s. found in the ectothermic vertebrates do not relate to taxonomic grouping.3. 3.|An inverse relationship exists between gut c.f. and body weight in ectotherms and also probably in mammals. This relationship is seen within an individual species rather than among species.4. 4.|Secondary intrinsic contractions occur regularly in gut of ectotherms and much less frequently in mammalian gut. In ectothermic vertebrates, these thermally sensitive gut contractions are often at higher frequency than major contractions at high gut temperatures but cease at the same minimum temperatures.5. 5.|Unlike all other species tested, fish (bullheads, I. nebulosus) gut contractions were not rhythmic although they were thermally sensitive.6. 6.|Activation energies for thermally sensitive gut contractions in mammals are consistent with most values rangign from 14.5-18.5 Kcal/M while activation energies for secondary contractions were much more variable with a range of 4.4-29.0 Kcal/M.7. 7.|In laboratory mice, c.f. and c. amplitude are unaffected by pH in any biologically significant manner. Additionally, t.s. of neonatal (4-24 days old) lab mice are indicative of endotherms and are only slightly lower than adult levels 4 days after birth.Peer Reviewedhttp://deepblue.lib.umich.edu/bitstream/2027.42/22943/1/0000510.pd
Repositioning the Catalytic Triad Aspartic Acid of Haloalkane Dehalogenase: Effects on Stability, Kinetics, and Structure
Haloalkane dehalogenase (DhlA) catalyzes the hydrolysis of haloalkanes via an alkyl-enzyme intermediate. The covalent intermediate, which is formed by nucleophilic substitution with Asp124, is hydrolyzed by a water molecule that is activated by His289. The role of Asp260, which is the third member of the catalytic triad, was studied by site-directed mutagenesis. Mutation of Asp260 to asparagine resulted in a catalytically inactive D260N mutant, which demonstrates that the triad acid Asp260 is essential for dehalogenase activity. Furthermore, Asp260 has an important structural role, since the D260N enzyme accumulated mainly in inclusion bodies during expression, and neither substrate nor product could bind in the active-site cavity. Activity for brominated substrates was restored to D260N by replacing Asn148 with an aspartic or glutamic acid. Both double mutants D260N+N148D and D260N+N148E had a 10-fold reduced kcat and 40-fold higher Km values for 1,2-dibromoethane compared to the wild-type enzyme. Pre-steady-state kinetic analysis of the D260N+N148E double mutant showed that the decrease in kcat was mainly caused by a 220-fold reduction of the rate of carbon-bromine bond cleavage and a 10-fold decrease in the rate of hydrolysis of the alkyl-enzyme intermediate. On the other hand, bromide was released 12-fold faster and via a different pathway than in the wild-type enzyme. Molecular modeling of the mutant showed that Glu148 indeed could take over the interaction with His289 and that there was a change in charge distribution in the tunnel region that connects the active site with the solvent. On the basis of primary structure similarity between DhlA and other α/β-hydrolase fold dehalogenases, we propose that a conserved acidic residue at the equivalent position of Asn148 in DhlA is the third catalytic triad residue in the latter enzymes.
The actinobacterial transcription factor RbpA binds to the principal sigma subunit of RNA polymerase
RbpA is a small non-DNA-binding transcription factor that associates with RNA polymerase holoenzyme and stimulates transcription in actinobacteria, including Streptomyces coelicolor and Mycobacterium tuberculosis. RbpA seems to show specificity for the vegetative form of RNA polymerase as opposed to alternative forms of the enzyme. Here, we explain the basis of this specificity by showing that RbpA binds directly to the principal σ subunit in these organisms, but not to more diverged alternative σ factors. Nuclear magnetic resonance spectroscopy revealed that, although differing in their requirement for structural zinc, the RbpA orthologues from S. coelicolor and M. tuberculosis share a common structural core domain, with extensive, apparently disordered, N- and C-terminal regions. The RbpA-σ interaction is mediated by the C-terminal region of RbpA and σ domain 2, and S. coelicolor RbpA mutants that are defective in binding σ are unable to stimulate transcription in vitro and are inactive in vivo. Given that RbpA is essential in M. tuberculosis and critical for growth in S. coelicolor, these data support a model in which RbpA plays a key role in the σ cycle in actinobacteria
In vitro transposition of ISY100, a bacterial insertion sequence belonging to the Tc1/mariner family
The Synechocystis sp. PCC6803 insertion sequence ISY100 (ISTcSa) belongs to the Tc1/mariner/IS630 family of transposable elements. ISY100 transposase was purified and shown to promote transposition in vitro. Transposase binds specifically to ISY100 terminal inverted repeat sequences via an N-terminal DNA-binding domain containing two helix–turn–helix motifs. Transposase is the only protein required for excision and integration of ISY100. Transposase made double-strand breaks on a supercoiled DNA molecule containing a mini-ISY100 transposon, cleaving exactly at the transposon 3′ ends and two nucleotides inside the 5′ ends. Cleavage of short linear substrates containing a single transposon end was less precise. Transposase also catalysed strand transfer, covalently joining the transposon 3′ end to the target DNA. When a donor plasmid carrying a mini-ISY100 was incubated with a target plasmid and transposase, the most common products were insertions of one transposon end into the target DNA, but insertions of both ends at a single target site could be recovered after transformation into Escherichia coli. Insertions were almost exclusively into TA dinucleotides, and the target TA was duplicated on insertion. Our results demonstrate that there are no fundamental differences between the transposition mechanisms of IS630 family elements in bacteria and Tc1/mariner elements in higher eukaryotes
A Revised Design for Microarray Experiments to Account for Experimental Noise and Uncertainty of Probe Response
Background
Although microarrays are analysis tools in biomedical research, they are known to yield noisy output that usually requires experimental confirmation. To tackle this problem, many studies have developed rules for optimizing probe design and devised complex statistical tools to analyze the output. However, less emphasis has been placed on systematically identifying the noise component as part of the experimental procedure. One source of noise is the variance in probe binding, which can be assessed by replicating array probes. The second source is poor probe performance, which can be assessed by calibrating the array based on a dilution series of target molecules. Using model experiments for copy number variation and gene expression measurements, we investigate here a revised design for microarray experiments that addresses both of these sources of variance.
Results
Two custom arrays were used to evaluate the revised design: one based on 25 mer probes from an Affymetrix design and the other based on 60 mer probes from an Agilent design. To assess experimental variance in probe binding, all probes were replicated ten times. To assess probe performance, the probes were calibrated using a dilution series of target molecules and the signal response was fitted to an adsorption model. We found that significant variance of the signal could be controlled by averaging across probes and removing probes that are nonresponsive or poorly responsive in the calibration experiment. Taking this into account, one can obtain a more reliable signal with the added option of obtaining absolute rather than relative measurements.
Conclusion
The assessment of technical variance within the experiments, combined with the calibration of probes allows to remove poorly responding probes and yields more reliable signals for the remaining ones. Once an array is properly calibrated, absolute quantification of signals becomes straight forward, alleviating the need for normalization and reference hybridizations
Alternate SlyA and H-NS nucleoprotein complexes control hlyE expression in Escherichia coli K-12
Haemolysin E is a cytolytic pore-forming toxin found in several Escherichia coli and Salmonella enterica strains. Expression of hlyE is repressed by the global regulator H-NS (histone-like nucleoid structuring protein), but can be activated by the regulator SlyA. Expression of a chromosomal hlyE–lacZ fusion in an E. coli slyA mutant was reduced to 60% of the wild-type level confirming a positive role for SlyA. DNase I footprint analysis revealed the presence of two separate SlyA binding sites, one located upstream, the other downstream of the hlyE transcriptional start site. These sites overlap AT-rich H-NS binding sites. Footprint and gel shift data showed that whereas H-NS prevented binding of RNA polymerase (RNAP) at the hlyE promoter (PhlyE), SlyA allowed binding of RNAP, but inhibited binding of H-NS. Accordingly, in vitro transcription analyses showed that addition of SlyA protein relieved H-NS-mediated repression of hlyE. Based on these observations a model for SlyA/H-NS regulation of hlyE expression is proposed in which the relative concentrations of SlyA and H-NS govern the nature of the nucleoprotein complexes formed at PhlyE. When H-NS is dominant RNAP binding is inhibited and hlyE expression is silenced; when SlyA is dominant H-NS binding is inhibited allowing RNAP access to the promoter facilitating hlyE transcription
Nutritional budgets in free flying birds: Cedar waxwings (Bombycilla cedrorum) feeding on washington hawthorn fruit (Crataegus phaenopyrum)
1. 1. Nutritional balances for calories, glucose, water, nitrogen, Na+, K+, Ca2+, and Mg2+ have been estimated for free-flying cedar waxwings feeding on Washington hawthorn fruits.2. 2. Birds assimilate 39.9 calories/fruit ( = 20.0% of available calories) and a net loss of 155mg of water/fruit.3. 3. Reducing sugars account for 74.5% of assimilated calories ( = 66.0% assimilation efficiency).4. 4. While feeding on these fruits, birds exhibit positive nitrogen and caloric balance, and negative Na+, K+, Mg2+, Ca2+, and water balances.Peer Reviewedhttp://deepblue.lib.umich.edu/bitstream/2027.42/27569/1/0000613.pd
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