Structures of oligomycin A and C structures of three isomeric octadecadienoic acids possessing divalent cation ionophoreticc activity : insecticidal components of dill and anise plants /

Carter, Guy Thomas,

January 1976

Thesis (Ph. D.)--University of Wisconsin--Madison, 1976. / Typescript. Vita. eContent provider-neutral record in process. Description based on print version record. Bibliography: leaves 170-172.

Oligomycin.

Chemical structures of oligomycins A and B

Prouty, Walter Francis,

January 1970

Thesis (Ph. D.)--University of Wisconsin--Madison, 1970. / Typescript. Vita. eContent provider-neutral record in process. Description based on print version record. Includes bibliographical references.

Oligomycin. Antibiotics.

Structural studies of Na'+K'+-ATPase

Carradus, Maria

January 2001

No description available.

572

Oligomycin; Rubidium

Chemistry of oligomycin B Localization of glycogen in the opacity characterizing decidualization in the cleared hamster uterus.

Foster, George Andrew,

January 1966

Thesis (Ph. D.)--University of Wisconsin, 1966. / "Localization of glycogen in the opacity characterizing decidualization in the cleared hamster uterus [by] G. A. Foster, Margaret Ward Orsini and F. M. Strong, reprinted from Proceedings of the Society for Experimental Biology and Medicine" inserted following leaf 214. Typescript. Vita. eContent provider-neutral record in process. Description based on print version record. Includes bibliography.

Oligomycin. Glycogen. Uterus Hamsters.

Isolation of antibiotic-resistant mutants and biochemical characterization of oligomycin resistance in Acanthamoeba castellanii /

Seilhammer, Jeffrey John,

January 1979

No description available.

Biology

Oligomycin

Acanthamoeba castellanii

Monitoring Dielectric Properties of Single MRC5 Cells and Oligomycin Treated Chinese Hamster Ovary Cells Using a Dielectrophoretic Cytometer

Saboktakin Rizi, Bahareh

17 September 2014

We have employed a differential detector combined with dielectrophoretic (DEP) translation in a microfluidic channel to monitor dielectric response of single cells and particularly to track phenomenon related to apoptosis. Two different cell lines were studied; Chinese hamster ovary cells (CHO) and MRC5 cells. Dielectric response was quantified by a factor called Force Index. Force Index was studied statistically to identify apoptotic subpopulations. Another direction of this work was to monitor changes in the cytoplasm conductivity following inhibition of mitochondrial ATP production by Oligomycin. To make the DEP response mostly sensitive to the cytoplasm conductivity, medium conductivity and DEP frequency were adjusted such that Clausius Mossotti factor and hence DEP response become less sensitive to cell radius. Chinese hamster ovary cells were used in this work and the impact of different concentrations of Oligomycin has been studied. We show that following exposure to Oligomycin at 8 μg/ml, cytoplasm conductivity drops. The majority of the changes takes place within one hour of exposure to the drug. Furthermore, double shell models has been used to estimate cytoplasm conductivity in a medium with conductivity of 0.42 S/m and the drop in the cytoplasm conductivity following treatment with Oligomycin was estimated to be ≈ 0.16 S/m. The magnitude of the decrease in the cytoplasm conductivity is evidence that Glycolysis is active as an energy production pathway within the cell. This approach can be used to quantify Glycolysis versus mitochondria ATP production which has an application in Warburg effect in cancer cells and monitoring bioprocesses.

Dielectrophoresis

Single cell analysis

Oligomycin

Cytoplasm conductivity

ATP inhibition

Chinese Hamster Ovary Cells

Oxidative Stress and Cell Death in Osmotically Swollen Glial Cells

Stuckey, Crystal Elaine

08 May 2008

No description available.

Cellular Biology

Microbiology

Neurology

C6

glia

DCFDA

hypoosmotic

ROS

ATP

cell death

NADPH oxidase

mitochondrial ETC

DPI

oligomycin

rotenone

Studium deficitu lidské F1Fo-ATPsyntázy / Human F1Fo-ATPsynthase deficiency

Suldovská, Sabina

January 2010

F1FO-ATPsynthase is a key enzyme in energy metabolism of the cell. Its deficit is caused usually by mutations in two structural genes MT-ATP6 and MT-ATP8 encoded by the mitochondrial DNA or in nuclear genes ATPAF2 and TMEM70 encoding the biogenesis factors and structural gene ATP5E. Deficiency of the F1FO-ATPsynthase leads to progressive and serious phenotype affecting organs with high energy demands. The first symptoms usually occurs in neonatal age and prognosis of the disease is fatal. Mutations in these genes result in both qualitative and quantitative defects of the F1FO-ATPsynthase. The study of molecular bases of mitochondrial disorders including F1FO-ATPsynthase deficiency uses large number of biochemical and molecular-genetic methods to determine a proper diagnosis which is essential for the symptomatic therapy and genetic counselling in affected families. The aim of the diploma thesis was to characterise the F1FO-ATPsynthase deficiency in isolated mitochondria from the lines of cultured cells by the determination oligomycin- sensitive ATP-hydrolytic activity of the F1FO-ATPsynthase, enzymatic activities of the respiratory chain complexes and to analyse changes in the steady-state levels of the representative subunits and whole complex of the F1FO-ATPsynthase in comparison with controls. 3...