A Bacillus anthracis-Based In Vitro System Supports Replication of Plasmid pXO2 as Well as Rolling-Circle-Replicating Plasmids

Translation of GCN4 mRNA is activated when yeast cells are grown under conditions of amino acid limitation. In this study, we established the conditions through which translation of the GCN4 mRNA could be activated in a homologous in vitro system. This activation paralleled the in vivo situation: it required the small open reading frames located in the 5' untranslated region of the GCN4 mRNA, and it was coupled with reduced rates of 43S preinitiation complex formation. Translational derepression in vitro was triggered by uncharged tRNA molecules, demonstrating that deacylated tRNAs are more proximal signals for translational activation of the GCN4 mRNA.

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Translational activation of GCN4 mRNA in a cell-free system is triggered by uncharged tRNAs.

Molecular and Cellular Biology ◽

10.1128/mcb.10.8.4375 ◽

1990 ◽

Vol 10 (8) ◽

pp. 4375-4378 ◽

Cited By ~ 7

Author(s):

G Krupitza ◽

G Thireos

Keyword(s):

Open Reading Frames ◽

Yeast Cells ◽

Free System ◽

In Vitro System ◽

A Cell ◽

Translational Activation ◽

Reading Frames ◽

Small Open Reading Frames

Translation of GCN4 mRNA is activated when yeast cells are grown under conditions of amino acid limitation. In this study, we established the conditions through which translation of the GCN4 mRNA could be activated in a homologous in vitro system. This activation paralleled the in vivo situation: it required the small open reading frames located in the 5' untranslated region of the GCN4 mRNA, and it was coupled with reduced rates of 43S preinitiation complex formation. Translational derepression in vitro was triggered by uncharged tRNA molecules, demonstrating that deacylated tRNAs are more proximal signals for translational activation of the GCN4 mRNA.

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Bacillus anthracis and Bacillus cereus PcrA Helicases Can Support DNA Unwinding and In Vitro Rolling-Circle Replication of Plasmid pT181 of Staphylococcus aureus

Journal of Bacteriology ◽

10.1128/jb.186.7.2195-2199.2004 ◽

2004 ◽

Vol 186 (7) ◽

pp. 2195-2199 ◽

Cited By ~ 27

Author(s):

Syam P. Anand ◽

Poulami Mitra ◽

Asma Naqvi ◽

Saleem A. Khan

Keyword(s):

Staphylococcus Aureus ◽

Bacillus Cereus ◽

Bacillus Anthracis ◽

Broad Host Range ◽

Gram Positive ◽

Rolling Circle ◽

Initiator Protein ◽

Gram Positive Bacteria ◽

Plasmid Pt181

ABSTRACT Replication of rolling-circle replicating (RCR) plasmids in gram-positive bacteria requires the unwinding of initiator protein-nicked plasmid DNA by the PcrA helicase. In this report, we demonstrate that heterologous PcrA helicases from Bacillus anthracis and Bacillus cereus are capable of unwinding Staphylococcus aureus plasmid pT181 from the initiator-generated nick and promoting in vitro replication of the plasmid. These helicases also physically interact with the RepC initiator protein of pT181. The ability of PcrA helicases to unwind noncognate RCR plasmids may contribute to the broad-host-range replication and dissemination of RCR plasmids in gram-positive bacteria.

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Differential stability of c-myc mRNAS in a cell-free system

Molecular and Cellular Biology ◽

10.1128/mcb.8.7.2860-2868.1988 ◽

1988 ◽

Vol 8 (7) ◽

pp. 2860-2868

Author(s):

R Pei ◽

K Calame

Keyword(s):

Full Length ◽

Free System ◽

In Vitro System ◽

Rapid Degradation ◽

Cell Free System ◽

Exon 1 ◽

A Cell ◽

The Stability

We have developed a simple cell-free system for studying the stability of different mRNAs in vitro. We demonstrate that the threefold greater stability in vivo of truncated c-myc mRNA (lacking exon 1) compared with that of full-length c-myc mRNA is maintained in our in vitro system. Chimeric mRNAs in which the first exon of c-myc was fused to immunoglobulin C alpha heavy chain or glyceraldehyde-3-phosphate dehydrogenase mRNAs were not rapidly degraded, demonstrating that c-myc exon 1 alone is not sufficient to tag mRNAs for rapid degradation. Competition experiments show that full-length c-myc mRNA is specifically recognized by a factor(s) responsible for its rapid degradation. This system will allow further characterization and purification of these factors.

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Cell-free reconstitution of vacuole membrane fragmentation reveals regulation of vacuole size and number by TORC1

Molecular Biology of the Cell ◽

10.1091/mbc.e11-08-0703 ◽

2012 ◽

Vol 23 (5) ◽

pp. 881-895 ◽

Cited By ~ 45

Author(s):

Lydie Michaillat ◽

Tonie Luise Baars ◽

Andreas Mayer

Keyword(s):

Copy Number ◽

Nutrient Restriction ◽

Lysosomal Hydrolases ◽

Gtp Hydrolysis ◽

Free System ◽

In Vitro System ◽

Vacuolar Compartment ◽

Vacuole Fusion ◽

A Cell

Size and copy number of organelles are influenced by an equilibrium of membrane fusion and fission. We studied this equilibrium on vacuoles—the lysosomes of yeast. Vacuole fusion can readily be reconstituted and quantified in vitro, but it had not been possible to study fission of the organelle in a similar way. Here we present a cell-free system that reconstitutes fragmentation of purified yeast vacuoles (lysosomes) into smaller vesicles. Fragmentation in vitro reproduces physiological aspects. It requires the dynamin-like GTPase Vps1p, V-ATPase pump activity, cytosolic proteins, and ATP and GTP hydrolysis. We used the in vitro system to show that the vacuole-associated TOR complex 1 (TORC1) stimulates vacuole fragmentation but not the opposing reaction of vacuole fusion. Under nutrient restriction, TORC1 is inactivated, and the continuing fusion activity then dominates the fusion/fission equilibrium, decreasing the copy number and increasing the volume of the vacuolar compartment. This result can explain why nutrient restriction not only induces autophagy and a massive buildup of vacuolar/lysosomal hydrolases, but also leads to a concomitant increase in volume of the vacuolar compartment by coalescence of the organelles into a single large compartment.

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Differential stability of c-myc mRNAS in a cell-free system.

Molecular and Cellular Biology ◽

10.1128/mcb.8.7.2860 ◽

1988 ◽

Vol 8 (7) ◽

pp. 2860-2868 ◽

Cited By ~ 35

Author(s):

R Pei ◽

K Calame

Keyword(s):

Full Length ◽

Free System ◽

In Vitro System ◽

Rapid Degradation ◽

Cell Free System ◽

Exon 1 ◽

A Cell ◽

The Stability

We have developed a simple cell-free system for studying the stability of different mRNAs in vitro. We demonstrate that the threefold greater stability in vivo of truncated c-myc mRNA (lacking exon 1) compared with that of full-length c-myc mRNA is maintained in our in vitro system. Chimeric mRNAs in which the first exon of c-myc was fused to immunoglobulin C alpha heavy chain or glyceraldehyde-3-phosphate dehydrogenase mRNAs were not rapidly degraded, demonstrating that c-myc exon 1 alone is not sufficient to tag mRNAs for rapid degradation. Competition experiments show that full-length c-myc mRNA is specifically recognized by a factor(s) responsible for its rapid degradation. This system will allow further characterization and purification of these factors.

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Natural 2′,5′-Phosphodiester Bonds Found at the Ligation Sites of Peach Latent Mosaic Viroid

Journal of Virology ◽

10.1128/jvi.75.1.19-25.2001 ◽

2001 ◽

Vol 75 (1) ◽

pp. 19-25 ◽

Cited By ~ 33

Author(s):

Fabien Côté ◽

Dominique Lévesque ◽

Jean-Pierre Perreault

Keyword(s):

Circular Rna ◽

Rolling Circle ◽

Phosphodiester Bonds ◽

Biological Importance ◽

Rolling Circle Mechanism ◽

Ligation Site

ABSTRACT Peach latent mosaic viroid (PLMVd) is a circular RNA pathogen that replicates in a DNA-independent fashion via a rolling circle mechanism. PLMVd has been shown to self-ligate in vitro primarily via the formation of 2′,5′-phosphodiester bonds; however, in vivo the occurrence and necessity of this nonenzymatic mechanism are not evident. Here, we unequivocally report the presence of 2′,5′-phosphodiester bonds at the ligation site of circular PLMVd strands isolated from infected peach leaves. These bonds serve to close the linear conformers (i.e., intermediates), yielding circular ones. Furthermore, these bonds are shown to stabilize the replicational circular templates, resulting in a significant advantage in terms of viroid viability. Although the mechanism responsible for the formation of these 2′,5′-phosphodiester bonds remains to be elucidated, a hypothesis describing in vivo nonenzymatic self-ligation is proposed. Most significantly, our results clearly show that 2′,5′-phosphodiester bonds are still present in nature and that they are of biological importance.

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Cross-talk between IRAK-4 and the NADPH oxidase1

Biochemical Journal ◽

10.1042/bj20061184 ◽

2007 ◽

Vol 403 (3) ◽

pp. 451-461 ◽

Cited By ~ 50

Author(s):

Sandrine Pacquelet ◽

Jennifer L. Johnson ◽

Beverly A. Ellis ◽

Agnieszka A. Brzezinska ◽

William S. Lane ◽

...

Keyword(s):

Protein Kinase ◽

Nadph Oxidase ◽

P38 Mapk ◽

Interleukin 1 ◽

Mitogen Activated Protein Kinase ◽

Free System ◽

Mitogen Activated Protein ◽

A Cell ◽

Tlr4 Activation

Exposure of neutrophils to LPS (lipopolysaccharide) triggers their oxidative response. However, the relationship between the signalling downstream of TLR4 (Toll-like receptor 4) after LPS stimulation and the activation of the oxidase remains elusive. Phosphorylation of the cytosolic factor p47phox is essential for activation of the NADPH oxidase. In the present study, we examined the hypothesis that IRAK-4 (interleukin-1 receptor-associated kinase-4), the main regulatory kinase downstream of TLR4 activation, regulates the NADPH oxidase through phosphorylation of p47phox. We show that p47phox is a substrate for IRAK-4. Unlike PKC (protein kinase C), IRAK-4 phosphorylates p47phox not only at serine residues, but also at threonine residues. Target residues were identified by tandem MS, revealing a novel threonine-rich regulatory domain. We also show that p47phox is phosphorylated in granulocytes in response to LPS stimulation. LPS-dependent phosphorylation of p47phox was enhanced by the inhibition of p38 MAPK (mitogen-activated protein kinase), confirming that the kinase operates upstream of p38 MAPK. IRAK-4-phosphorylated p47phox activated the NADPH oxidase in a cell-free system, and IRAK-4 overexpression increased NADPH oxidase activity in response to LPS. We have shown that endogenous IRAK-4 interacts with p47phox and they co-localize at the plasma membrane after LPS stimulation, using immunoprecipitation assays and immunofluorescence microscopy respectively. IRAK-4 was activated in neutrophils in response to LPS stimulation. We found that Thr133, Ser288 and Thr356, targets for IRAK-4 phosphorylation in vitro, are also phosphorylated in endogenous p47phox after LPS stimulation. We conclude that IRAK-4 phosphorylates p47phox and regulates NADPH oxidase activation after LPS stimulation.

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Use of an in Vitro Protein Synthesizing System to Test the Mode of Action of Chloracetamides

Weed Science ◽

10.1017/s0043174500055417 ◽

1980 ◽

Vol 28 (3) ◽

pp. 334-340 ◽

Cited By ~ 26

Author(s):

Luanne M. Deal ◽

J. T. Reeves ◽

B. A. Larkins ◽

F. D. Hess

Keyword(s):

Protein Synthesis ◽

Sand Culture ◽

Leucine Incorporation ◽

Insoluble Protein ◽

In Vitro System ◽

A Cell ◽

Protein Incorporation ◽

Vitro Protein

The effects of chloracetamides on protein synthesis were studied both in vivo and in vitro. Four chloracetamide herbicides, alachlor [2-chloro-2′,6′-diethyl-N-(methoxymethyl)acetanilide], metolachlor [2-chloro-N-(2-ethyl-6-methylphenyl)-N-(2-methoxy-1-methylethyl)acetamide], CDAA (N–N-diallyl-2-chloroacetamide), and propachlor (2-chloro-N-isopropylacetanilide) were tested for inhibition of [3H]-leucine incorporation into protein. Incorporation of3H-leucine into trichloroacetic acid (TCA)-insoluble protein was inhibited in oat (Avena sativaL. ‘Victory’) seedlings grown in sand culture and treated 12 h at 1 × 10−4M with these chloracetamides. The herbicides were also tested in a cell-free protein synthesizing system containing polyribosomes purified from oat root cytoplasm. These herbicides had no effect on the rates of polypeptide elongation nor on the synthesis of specific polypeptides when herbicides (1 × 10−4M) were added directly to the system. Polypeptide formation was inhibited 89% when 1 × 10−4M cycloheximide was added during translation. Cytoplasmic polyribosomes were isolated from oat roots treated 12 h with 1 × 10−4M herbicide. Translation rates and products were not altered when these polyribosomes were added to the in vitro system. Protein synthesis is inhibited when tested in an in vivo system; however, the inhibition does not occur during the translation of mRNA into protein.

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Efficacy of a Potential Trivalent Vaccine Based on Hc Fragments of Botulinum Toxins A, B, and E Produced in a Cell-Free Expression System

Clinical and Vaccine Immunology ◽

10.1128/cvi.00496-09 ◽

2010 ◽

Vol 17 (5) ◽

pp. 784-792 ◽

Cited By ~ 34

Author(s):

R. Zichel ◽

A. Mimran ◽

A. Keren ◽

A. Barnea ◽

I. Steinberger-Levy ◽

...

Keyword(s):

Expression System ◽

Free Expression ◽

Enzyme Linked Immunosorbent Assay ◽

High Dose ◽

Botulinum Toxins ◽

Free System ◽

Toxin Complex ◽

A Cell ◽

Cell Free Expression System

ABSTRACT Botulinum toxins produced by the anaerobic bacterium Clostridium botulinum are the most potent biological toxins in nature. Traditionally, people at risk are immunized with a formaldehyde-inactivated toxin complex. Second generation vaccines are based on the recombinant carboxy-terminal heavy-chain (Hc) fragment of the neurotoxin. However, the materialization of this approach is challenging, mainly due to the high AT content of clostridial genes. Herein, we present an alternative strategy in which the native genes encoding Hc proteins of botulinum toxins A, B, and E were used to express the recombinant Hc fragments in a cell-free expression system. We used the unique property of this open system to introduce different combinations of chaperone systems, protein disulfide isomerase (PDI), and reducing/oxidizing environments directly to the expression reaction. Optimized expression conditions led to increased production of soluble Hc protein, which was successfully scaled up using a continuous exchange (CE) cell-free system. Hc proteins were produced at a concentration of more than 1 mg/ml and purified by one-step Ni+ affinity chromatography. Mice immunized with three injections containing 5 μg of any of the in vitro-expressed, alum-absorbed, Hc vaccines generated a serum enzyme-linked immunosorbent assay (ELISA) titer of 105 against the native toxin complex, which enabled protection against a high-dose toxin challenge (103 to 106 mouse 50% lethal dose [MsLD50]). Finally, immunization with a trivalent HcA, HcB, and HcE vaccine protected mice against the corresponding trivalent 105 MsLD50 toxin challenge. Our results together with the latest developments in scalability of the in vitro protein expression systems offer alternative routes for the preparation of botulinum vaccine.

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