PROBLEMS ASSOCIATED WITH THE USE OF THE EXPOSED PLATINUM ELECTRODE FOR MEASURING OXYGEN TENSION IN VIVO

The equation governing the distribution of oxygen around a stationary exposed platinum electrode was solved for the size of electrode used and for a number of different times. In protein solutions the oxygen polarogram could be satisfactorily monitored by measuring the diffusion current at −0.6 and −0.7 volts. After using the platinum electrode in solutions containing protein it was found necessary and sufficient to clean it in acid dichromate solution followed by neutralization in a buffer solution. This procedure reproduced the original diffusion current. In solutions containing heterogeneities with small coefficients of oxygen diffusion, the electrode current was found to be less than when the heterogeneities were not present.

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NK cell activation through the NKG2D ligand MULT-1 is selectively prevented by the glycoprotein encoded by mouse cytomegalovirus gene m145

Journal of Experimental Medicine ◽

10.1084/jem.20041617 ◽

2005 ◽

Vol 201 (2) ◽

pp. 211-220 ◽

Cited By ~ 115

Author(s):

Astrid Krmpotic ◽

Milena Hasan ◽

Andrea Loewendorf ◽

Tanja Saulig ◽

Anne Halenius ◽

...

Keyword(s):

Cell Activation ◽

Nk Cell ◽

Surface Expression ◽

Viral Gene ◽

Nkg2d Ligand ◽

Mouse Cytomegalovirus ◽

Mcmv Infection ◽

Viral Survival ◽

Necessary And Sufficient

The NK cell–activating receptor NKG2D interacts with three different cellular ligands, all of which are regulated by mouse cytomegalovirus (MCMV). We set out to define the viral gene product regulating murine UL16-binding protein-like transcript (MULT)-1, a newly described NKG2D ligand. We show that MCMV infection strongly induces MULT-1 gene expression, but surface expression of this glycoprotein is nevertheless completely abolished by the virus. Screening a panel of MCMV deletion mutants defined the gene m145 as the viral regulator of MULT-1. The MCMV m145-encoded glycoprotein turned out to be necessary and sufficient to regulate MULT-1 by preventing plasma membrane residence of MULT-1. The importance of MULT-1 in NK cell regulation in vivo was confirmed by the attenuating effect of the m145 deletion that was lifted after NK cell depletion. Our findings underline the significance of escaping MULT-1/NKG2D signaling for viral survival and maintenance.

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Biological modification in air-cathode microbial fuel cell: Effect on oxygen diffusion, current generation and wastewater degradation

Chemosphere ◽

10.1016/j.chemosphere.2021.131243 ◽

2021 ◽

pp. 131243

Author(s):

Ambika Arkatkar ◽

Arvind Kumar Mungray ◽

Preeti Sharma

Keyword(s):

Fuel Cell ◽

Microbial Fuel Cell ◽

Oxygen Diffusion ◽

Diffusion Current ◽

Air Cathode ◽

Current Generation ◽

Biological Modification

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In vivo analysis of DNA-protein interactions on the human erythropoietin enhancer.

Molecular and Cellular Biology ◽

10.1128/mcb.17.2.851 ◽

1997 ◽

Vol 17 (2) ◽

pp. 851-856 ◽

Cited By ~ 18

Author(s):

B Hu ◽

E Wright ◽

L Campbell ◽

K L Blanchard

Keyword(s):

Oxygen Tension ◽

Protein Interactions ◽

Proximal Promoter ◽

Low Oxygen ◽

Initiation Rate ◽

Cobalt Exposure ◽

In Cells ◽

Dna Protein Interactions

The erythropoietin (EPO) gene is one of the best examples of a mammalian gene controlled by oxygen tension. The DNA elements responsible for hypoxia-induced transcription consist of a short region of the proximal promoter and a <50-bp 3' enhancer. The elements act cooperatively to increase the transcriptional initiation rate approximately 100-fold in response to low oxygen tension in Hep3B cells. Two distinct types of transactivating proteins have been demonstrated to bind the response elements in the human EPO enhancer in vitro: one shows hypoxia-inducible DNA binding activity, while the other activity binds DNA under normoxic and hypoxic conditions. We have investigated the DNA-protein interactions on the human EPO enhancer in living tissue culture cells that produce EPO in a regulated fashion (Hep3B) and in cells that do not express EPO under any conditions tested (HeLa). We have identified in vivo DNA-protein interactions on the control elements in the human EPO enhancer by ligation-mediated PCR technology. We show that the putative protein binding sites in the EPO enhancer are occupied in vivo under conditions of normoxia, hypoxia, and cobalt exposure in EPO-producing cells. These sites are not occupied in cells that do not produce EPO. We also provide evidence for a conformational change in the topography of the EPO enhancer in response to hypoxia and cobalt exposure.

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The ER–Golgi intermediate compartment is a key membrane source for the LC3 lipidation step of autophagosome biogenesis

eLife ◽

10.7554/elife.00947 ◽

2013 ◽

Vol 2 ◽

Cited By ~ 226

Author(s):

Liang Ge ◽

David Melville ◽

Min Zhang ◽

Randy Schekman

Keyword(s):

Autophagosome Formation ◽

Functional Studies ◽

A Cell ◽

Intermediate Compartment ◽

Membrane Isolation ◽

Necessary And Sufficient ◽

Organelle Membrane ◽

Catabolic Process

Autophagy is a catabolic process for bulk degradation of cytosolic materials mediated by double-membraned autophagosomes. The membrane determinant to initiate the formation of autophagosomes remains elusive. Here, we establish a cell-free assay based on LC3 lipidation to define the organelle membrane supporting early autophagosome formation. In vitro LC3 lipidation requires energy and is subject to regulation by the pathways modulating autophagy in vivo. We developed a systematic membrane isolation scheme to identify the endoplasmic reticulum–Golgi intermediate compartment (ERGIC) as a primary membrane source both necessary and sufficient to trigger LC3 lipidation in vitro. Functional studies demonstrate that the ERGIC is required for autophagosome biogenesis in vivo. Moreover, we find that the ERGIC acts by recruiting the early autophagosome marker ATG14, a critical step for the generation of preautophagosomal membranes.

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Diabetes increases stiffness of live cardiomyocytes measured by atomic force microscopy nanoindentation

AJP Cell Physiology ◽

10.1152/ajpcell.00192.2013 ◽

2014 ◽

Vol 307 (10) ◽

pp. C910-C919 ◽

Cited By ~ 22

Author(s):

Juan C. Benech ◽

Nicolás Benech ◽

Ana I. Zambrana ◽

Inés Rauschert ◽

Verónica Bervejillo ◽

...

Keyword(s):

Atomic Force Microscopy ◽

Physiological Condition ◽

Diabetic Mice ◽

Cell Nuclei ◽

Buffer Solution ◽

Isolated Cardiomyocytes ◽

Force Microscopy ◽

Atomic Force ◽

Myocardial Fibers

Stiffness of live cardiomyocytes isolated from control and diabetic mice was measured using the atomic force microscopy nanoindentation method. Type 1 diabetes was induced in mice by streptozotocin administration. Histological images of myocardium from mice that were diabetic for 3 mo showed disorderly lineup of myocardial cells, irregularly sized cell nuclei, and fragmented and disordered myocardial fibers with interstitial collagen accumulation. Phalloidin-stained cardiomyocytes isolated from diabetic mice showed altered (i.e., more irregular and diffuse) actin filament organization compared with cardiomyocytes from control mice. Sarco/endoplasmic reticulum Ca2+-ATPase (SERCA2a) pump expression was reduced in homogenates obtained from the left ventricle of diabetic animals compared with age-matched controls. The apparent elastic modulus (AEM) for live control or diabetic isolated cardiomyocytes was measured using the atomic force microscopy nanoindentation method in Tyrode buffer solution containing 1.8 mM Ca2+ and 5.4 mM KCl (physiological condition), 100 nM Ca2+ and 5.4 mM KCl (low extracellular Ca2+ condition), or 1.8 mM Ca2+ and 140 mM KCl (contraction condition). In the physiological condition, the mean AEM was 112% higher for live diabetic than control isolated cardiomyocytes (91 ± 14 vs. 43 ± 7 kPa). The AEM was also significantly higher in diabetic than control cardiomyocytes in the low extracellular Ca2+ and contraction conditions. These findings suggest that the material properties of live cardiomyocytes were affected by diabetes, resulting in stiffer cells, which very likely contribute to high diastolic LV stiffness, which has been observed in vivo in some diabetes mellitus patients.

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Reversible neutralization by congo red of the anthracidal power of serum

Journal of Hygiene ◽

10.1017/s002217240003518x ◽

1937 ◽

Vol 37 (3) ◽

pp. 471-473 ◽

Cited By ~ 1

Author(s):

J. Gordon ◽

N. Wood

Keyword(s):

Guinea Pig ◽

Congo Red ◽

Inhibitory Action ◽

Protein Solutions ◽

Haemolytic Activity ◽

In Vitro Experiments ◽

Serum Complement ◽

Destructive Effect

In earlier papers (Gordon, 1930) it was shown that congo red has an inactivating effect on serum complement, both haemolytic and bactericidal, and that this effect can be reversed by treating the serum and congo red mixture with charcoal, the charcoal removing the congo red and leaving the complement active again. A similar reversal of inactivation is obtained by using instead of the charcoal, heated serum (55° C. for 30 min.) or protein solutions. Later (Gordon, 1931), it was shown that congo red had an inactivating effect on the haemolysins of Streptococcus haemolyticus and B. welchii. The reversibility of this effect was not so easy to demonstrate as with complement. Charcoal had a destructive effect on the haemolysins and so could not be used. It was found, however, that when the concentration of congo red was just sufficient to neutralize the streptococcal haemolysin, the addition of cuprammonium artificial silk adsorbed the congo red and liberated the haemolysin. In the case of B. welchii this method of reversal was not suitable, as the artificial silk had a destructive effect on the haemolysin. Instead, reversibility was demonstrated by adding ox serum to the mixture of congo red and haemolysin. This brought about a redistribution of the congo red between the ox serum and the haemolysin and if the amount of congo red used had been only just sufficient to neutralize the haemolysin of B. welchii, then the haemolytic activity could again be demonstrated. Gordon and Robson (1933) showed that congo red interfered with the anaphylactic reaction tested both in vivo and in vitro, the guinea-pig uterus being used in the in vitro experiments, in which the inhibitory action of the dye was shown to be reversible. It was suggested that the congo red interfered with the entrance of antigen into the cell.

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Engineered Biosynthesis of a Novel Amidated Polyketide, Using the Malonamyl-Specific Initiation Module from the Oxytetracycline Polyketide Synthase

Applied and Environmental Microbiology ◽

10.1128/aem.72.4.2573-2580.2006 ◽

2006 ◽

Vol 72 (4) ◽

pp. 2573-2580 ◽

Cited By ~ 83

Author(s):

Wenjun Zhang ◽

Brian D. Ames ◽

Shiou-Chuan Tsai ◽

Yi Tang

Keyword(s):

Polyketide Synthase ◽

Major Product ◽

Polyketide Synthases ◽

Type Ii ◽

Streptomyces Rimosus ◽

Aromatic Polyketides ◽

Starter Unit ◽

Necessary And Sufficient ◽

Bacterial Type

ABSTRACT Tetracyclines are aromatic polyketides biosynthesized by bacterial type II polyketide synthases (PKSs). Understanding the biochemistry of tetracycline PKSs is an important step toward the rational and combinatorial manipulation of tetracycline biosynthesis. To this end, we have sequenced the gene cluster of oxytetracycline (oxy and otc genes) PKS genes from Streptomyces rimosus. Sequence analysis revealed a total of 21 genes between the otrA and otrB resistance genes. We hypothesized that an amidotransferase, OxyD, synthesizes the malonamate starter unit that is a universal building block for tetracycline compounds. In vivo reconstitution using strain CH999 revealed that the minimal PKS and OxyD are necessary and sufficient for the biosynthesis of amidated polyketides. A novel alkaloid (WJ35, or compound 2) was synthesized as the major product when the oxy-encoded minimal PKS, the C-9 ketoreductase (OxyJ), and OxyD were coexpressed in CH999. WJ35 is an isoquinolone compound derived from an amidated decaketide backbone and cyclized with novel regioselectivity. The expression of OxyD with a heterologous minimal PKS did not afford similarly amidated polyketides, suggesting that the oxy-encoded minimal PKS possesses novel starter unit specificity.

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CATHETER-TIP TRANSDUCER FOR CONTINUOUS IN-VIVO MEASUREMENT OF OXYGEN TENSION

The Lancet ◽

10.1016/s0140-6736(71)91451-6 ◽

1971 ◽

Vol 297 (7706) ◽

pp. 952-953

Author(s):

D KEY

Keyword(s):

Oxygen Tension ◽

In Vivo Measurement ◽

Catheter Tip

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The Myosin IXb Motor Activity Targets the Myosin IXb RhoGAP Domain as Cargo to Sites of Actin Polymerization

Molecular Biology of the Cell ◽

10.1091/mbc.e06-08-0771 ◽

2007 ◽

Vol 18 (4) ◽

pp. 1507-1518 ◽

Cited By ~ 44

Author(s):

Frank van den Boom ◽

Heiko Düssmann ◽

Katharina Uhlenbrock ◽

Marouan Abouhamed ◽

Martin Bähler

Keyword(s):

Motor Activity ◽

Actin Polymerization ◽

Fluorescence Recovery After Photobleaching ◽

Rho Gtpase ◽

Tail Region ◽

Lysine Residues ◽

Motor Region ◽

Necessary And Sufficient ◽

Loop 2

Myosin IXb (Myo9b) is a single-headed processive myosin that exhibits Rho GTPase-activating protein (RhoGAP) activity in its tail region. Using live cell imaging, we determined that Myo9b is recruited to extending lamellipodia, ruffles, and filopodia, the regions of active actin polymerization. A functional motor domain was both necessary and sufficient for targeting Myo9b to these regions. The head domains of class IX myosins comprise a large insertion in loop2. Deletion of the large Myo9b head loop 2 insertion abrogated the enrichment in extending lamellipodia and ruffles, but enhanced significantly the enrichment at the tips of filopodia and retraction fibers. The enrichment in the tips of filopodia and retraction fibers depended on four lysine residues C-terminal to the loop 2 insertion and the tail region. Fluorescence recovery after photobleaching and photoactivation experiments in lamellipodia revealed that the dynamics of Myo9b was comparable to that of actin. The exchange rates depended on the Myo9b motor region and motor activity, and they were also dependent on the turnover of F-actin. These results demonstrate that Myo9b functions as a motorized RhoGAP molecule in regions of actin polymerization and identify Myo9b head sequences important for in vivo motor properties.

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