386 research outputs found
Sliding Columnar Phase of DNA-Lipid Complexes
We introduce a simple model for DNA-cationic-lipid complexes in which
galleries between planar bilayer lipid lamellae contain DNA 2D smectic lattices
that couple orientationally and positionally to lattices in neighboring
galleries. We identify a new equilibrium phase in which there are long-range
orientational but not positional correlations between DNA lattices. We discuss
properties of this new phase such as its X-ray structure factor S(r), which
exhibits unusual exp(- const.ln^2 r) behavior as a function of in-plane
separation r.Comment: This file contains 4 pages of double column text and one postscript
figure. This version includes interactions between dislocations in a given
gallery and presents an improved estimate of the decoupling temperature. It
is the published versio
Elastic properties of grafted microtubules
We use single-particle tracking to study the elastic properties of single
microtubules grafted to a substrate. Thermal fluctuations of the free
microtubule's end are recorded, in order to measure position distribution
functions from which we calculate the persistence length of microtubules with
contour lengths between 2.6 and 48 micrometers. We find the persistence length
to vary by more than a factor of 20 over the total range of contour lengths.
Our results support the hypothesis that shearing between protofilaments
contributes significantly to the mechanics of microtubules.Comment: 9 pages, 3 figure
Structural Properties of the Sliding Columnar Phase in Layered Liquid Crystalline Systems
Under appropriate conditions, mixtures of cationic and neutral lipids and DNA
in water condense into complexes in which DNA strands form local 2D smectic
lattices intercalated between lipid bilayer membranes in a lamellar stack.
These lamellar DNA-cationic-lipid complexes can in principle exhibit a variety
of equilibrium phases, including a columnar phase in which parallel DNA strands
from a 2D lattice, a nematic lamellar phase in which DNA strands align along a
common direction but exhibit no long-range positional order, and a possible new
intermediate phase, the sliding columnar (SC) phase, characterized by a
vanishing shear modulus for relative displacement of DNA lattices but a
nonvanishing modulus for compressing these lattices. We develop a model capable
of describing all phases and transitions among them and use it to calculate
structural properties of the sliding columnar phase. We calculate displacement
and density correlation functions and x-ray scattering intensities in this
phase and show, in particular, that density correlations within a layer have an
unusual dependence on separation r. We
investigate the stability of the SC phase with respect to shear couplings
leading to the columnar phase and dislocation unbinding leading to the lamellar
nematic phase. For models with interactions only between nearest neighbor
planes, we conclude that the SC phase is not thermodynamically stable.
Correlation functions in the nematic lamellar phase, however, exhibit SC
behavior over a range of length scalesComment: 28 pages, 4 figure
Contribution of noncanonical antigens to virulence and adaptive immunity in human infection with enterotoxigenic E. coli
Enterotoxigenic Escherichia coli (ETEC) contributes significantly to the substantial burden of infectious diarrhea among children living in low- and middle-income countries. In the absence of a vaccine for ETEC, children succumb to acute dehydration as well as nondiarrheal sequelae related to these infections, including malnutrition. The considerable diversity of ETEC genomes has complicated canonical vaccine development approaches defined by a subset of ETEC pathovar-specific antigens known as colonization factors (CFs). To identify additional conserved immunogens unique to this pathovar, we employed an āopen-apertureā approach to capture all potential conserved ETEC surface antigens, in which we mined the genomic sequences of 89 ETEC isolates, bioinformatically selected potential surface-exposed pathovar-specific antigens conserved in more than 40% of the genomes (nā=ā118), and assembled the representative proteins onto microarrays, complemented with known or putative colonization factor subunit molecules (nā=ā52) and toxin subunits. These arrays were then used to interrogate samples from individuals with acute symptomatic ETEC infections. Surprisingly, in this approach, we found that immune responses were largely constrained to a small number of antigens, including individual colonization factor antigens and EtpA, an extracellular adhesin. In a Bangladeshi cohort of naturally infected children <2āyears of age, both EtpA and a second antigen, EatA, elicited significant serologic responses that were associated with protection from symptomatic illness. In addition, children infected with ETEC isolates bearing either etpA or eatA genes were significantly more likely to develop symptomatic disease. These studies support a role for antigens not presently targeted by vaccines (noncanonical) in virulence and the development of adaptive immune responses during ETEC infections. These findings may inform vaccine design efforts to complement existing approaches
Genomic Organization, Splice Variants and Expression of CGMl, a CD66-related Member of the Carcinoembryonic Antigen Gene Family
The tumor marker carcinoembryonic antigen (CEA) belongs to a family of proteins which are composed of one immunogiobulin variable domain and a varying number of immunoglobulin constant-like domains. Most of the membrane-bound members, which are anchored either by a glycosylphosphatidylinositol moiety or a transmembrane domain, have been shown to convey cell adhesion in vitro. Here we describe two splice variants of CGMI. a transmembrane member of the CEA family without immunoglobulin constant.like domains. CGM1a and CGM1c contain cytopiasmic domains of 71 and 31 amino acids, respectively, The cytoplasmic region of CGM1a is encoded by four exons (Cyt1-Cyt4). Differential splicing of the Cyt1 exon (53 bp)..
Identification of the Feline Humoral Immune Response to Bartonella henselae Infection by Protein Microarray
Background: Bartonella henselae is the zoonotic agent of cat scratch disease and causes potentially fatal infections in immunocompromised patients. Understanding the complex interactions between the hostās immune system and bacterial pathogens is central to the field of infectious diseases and to the development of effective diagnostics and vaccines. Methodology: We report the development of a microarray comprised of proteins expressed from 96 % (1433/1493) of the predicted ORFs encoded by the genome of the zoonotic pathogen Bartonella henselae. The array was probed with a collection of 62 uninfected, 62 infected, and 8 āāspecific-pathogen freeā ā naĆÆve cat sera, to profile the antibody repertoire elicited during natural Bartonella henselae infection. Conclusions: We found that 7.3 % of the B. henselae proteins on the microarray were seroreactive and that seroreactivity was not evenly distributed between predicted protein function or subcellular localization. Membrane proteins were significantly most likely to be seroreactive, although only 23 % of the membrane proteins were reactive. Conversely, we found that proteins involved in amino acid transport and metabolism were significantly underrepresented and did not contain any seroreactive antigens. Of all seroreactive antigens, 52 were differentially reactive with sera from infected cats, and 53 were equally reactive with sera from infected and uninfected cats. Thirteen of the seroreactive antigens were found to be differentially seroreactive between B. henselae type I and type II. Based on these results, we developed a classifier algorith
A practical device for pinpoint delivery of molecules into multiple neurons in culture
We have developed a device for pinpoint delivery of chemicals, proteins, and nucleic acids into cultured cells. The principle underlying the technique is the flow of molecules from the culture medium into cells through a rupture in the plasma membrane made by a needle puncture. DNA transfection is achieved by stabbing the needle tip into the nucleus. The CellBee device can be attached to any inverted microscope, and molecular delivery can be coupled with conventional live cell imaging. Because the position of the needle relative to the targeted cultured cells is computer-controlled, efficient delivery of molecules such as rhodamine into as many as 100 HeLa cells can be completed in 10Ā min. Moreover, specific target cells within a single dish can be transfected with multiple DNA constructs by simple changes of culture medium containing different plasmids. In addition, the nano-sized needle tip enables gentle molecular delivery, minimizing cell damage. This method permits DNA transfection into specific hippocampal neurons without disturbing neuronal circuitry established in culture
Domain formation in DODABācholesterol mixed systems monitored via nile red anisotropy
The effect of the cholesterol (Ch) on liposomes composed of the cationic lipid dioctadecyldimethylammonium bromide (DODAB) was assessed by studying both the steady-state and time-resolved fluorescence anisotropy of the dye Nile Red. The information obtained combined with analysis of the steady-state emission and luorescence lifetime of Nile Red (NR) for different cholesterol concentrations (5ā50%) elucidated the presence of ācondensed complexesā and cholesterol-rich domains in these mixed systems. The steady-state fluorescence spectra were decomposed into the sum of two lognormal emissions, emanating from two different states, and the effect of temperature on the anisotropy decay of Nile Red for different cholesterol concentrations was observed. At room temperature, the time-resolved anisotropy decays are indicative of NR being relatively immobile (manifest by a high rā value). At higher temperature, rotational times ca. 1 ns were obtained throughout and a trend in increasing hindrance was seen with increase of Ch content
Systems Biology Approach Predicts Antibody Signature Associated with Brucella melitensis Infection in Humans
A complete understanding of the factors that determine selection of antigens recognized by the humoral immune response following infectious agent challenge is lacking. Here we illustrate a systems biology approach to identify the antibody signature associated with Brucella melitensis (Bm) infection in humans and predict proteomic features of serodiagnostic antigens. By taking advantage of a full proteome microarray expressing previously cloned 1406 and newly cloned 1640 Bm genes, we were able to identify 122 immunodominant antigens and 33 serodiagnostic antigens. The reactive antigens were then classified according to annotated functional features (COGs), computationally predicted features (e.g., subcellular localization, physical properties), and protein expression estimated by mass spectrometry (MS). Enrichment analyses indicated that membrane association and secretion were significant enriching features of the reactive antigens, as were proteins predicted to have a signal peptide, a single transmembrane domain, and outer membrane or periplasmic location. These features accounted for 67% of the serodiagnostic antigens. An overlay of the seroreactive antigen set with proteomic data sets generated by MS identified an additional 24%, suggesting that protein expression in bacteria is an additional determinant in the induction of Brucella-specific antibodies. This analysis indicates that one-third of the proteome contains enriching features that account for 91% of the antigens recognized, and after B. melitensis infection the immune system develops significant antibody titers against 10% of the proteins with these enriching features. This systems biology approach provides an empirical basis for understanding the breadth and specificity of the immune response to B. melitensis and a new framework for comparing the humoral responses against other microorganisms
Nucleofection induces non-specific changes in the metabolic activity of transfected cells
Transfection has become an everyday technique widely used for functional studies in living cells. The choice of the particular transfection method is usually determined by its efficiency and toxicity, and possible functional consequences specific to the method used are normally overlooked. We describe here that nucleofection, a method increasingly used because of its convenience and high efficiency, increases the metabolic rate of some cancer cells, which can be misleading when used as a measure of proliferation. Moreover, nucleofection can alter the subcellular expression pattern of the transfected protein. These undesired effects are independent of the transfected nucleic acid, but depend on the particular cell line used. Therefore, the interpretation of functional data using this technology requires further controls and caution
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