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2. Noninvasive magnetic resonance spectroscopic pharmacodynamic markers of a novel histone deacetylase inhibitor, LAQ824, in human colon carcinoma cells and xenografts.

Author

Chung YL, Troy H, Kristeleit R, Aherne W, Jackson LE, Atadja P, Griffiths JR, Judson IR, Workman P, Leach MO, and Beloueche-Babari M

Subjects
Acetylation, Animals, Blotting, Western, Cell Cycle drug effects, Cell Proliferation drug effects, Colonic Neoplasms enzymology, Colonic Neoplasms pathology, Disease Models, Animal, Enzyme Inhibitors pharmacology, HT29 Cells, Histones metabolism, Humans, Immunoenzyme Techniques, Male, Mice, Mice, Nude, Phosphorus Isotopes, Phosphorylcholine metabolism, Tumor Cells, Cultured, Vorinostat, Xenograft Model Antitumor Assays, Biomarkers, Tumor metabolism, Colonic Neoplasms drug therapy, Histone Deacetylase Inhibitors, Hydroxamic Acids therapeutic use, Nuclear Magnetic Resonance, Biomolecular methods
Abstract

The aim of this work was to use phosphorus magnetic resonance spectroscopy ((31)P MRS) to investigate the pharmacodynamic effects of LAQ824, a histone deacetylase (HDAC) inhibitor. Human HT29 colon carcinoma cells were examined by (31)P MRS after treatment with LAQ824 and another HDAC inhibitor, suberoylanilide hydroxamic acid. HT29 xenografts and tumor extracts were also examined using (31)P MRS, pre- and post-LAQ824 treatment. Histone H3 acetylation was determined using Western blot analysis, and tumor microvessel density by immunohistochemical staining of CD31. Phosphocholine showed a significant increase in HT29 cells after treatment with LAQ824 and suberoylanilide hydroxamic acid. In vivo, the ratio of phosphomonoester/total phosphorus (TotP) signal was significantly increased in LAQ824-treated HT29 xenografts, and this ratio was inversely correlated with changes in tumor volume. Statistically significant decreases in intracellular pH, beta-nucleoside triphosphate (beta-NTP)/TotP, and beta-NTP/inorganic phosphate (Pi) and an increase in Pi/TotP were also seen in LAQ824-treated tumors. Tumor extracts showed many significant metabolic changes after LAQ824 treatment, in parallel with increased histone acetylation and decreased microvessel density. Treatment with LAQ824 resulted in altered phospholipid metabolism and compromised tumor bioenergetics. The phosphocholine and phosphomonoester increases may have the potential to act as pharmacodynamic markers for noninvasively monitoring tumor response after treatment with LAQ824 or other HDAC inhibitors.

Published
2008
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3. A prospective, blinded analysis of thymidylate synthase and p53 expression as prognostic markers in the adjuvant treatment of colorectal cancer.

Author

Popat S, Chen Z, Zhao D, Pan H, Hearle N, Chandler I, Shao Y, Aherne W, and Houlston R

Subjects
Colorectal Neoplasms drug therapy, Colorectal Neoplasms enzymology, Female, Humans, Immunohistochemistry, Male, Middle Aged, Prognosis, Prospective Studies, Antimetabolites, Antineoplastic therapeutic use, Biomarkers, Tumor metabolism, Chemotherapy, Adjuvant, Colorectal Neoplasms metabolism, Fluorouracil therapeutic use, Thymidylate Synthase metabolism, Tumor Suppressor Protein p53 metabolism
Abstract

Background: Despite previous studies, uncertainty has persisted about the role of thymidylate synthase (TS) and p53 status as markers of prognosis in colorectal cancer (CRC)., Patients and Methods: A total of 967 patients accrued to a large adjuvant trial in CRC were included in a prospectively planned molecular substudy, and of them, 59% had rectal cancer and about 90% received adjuvant chemotherapy (either systemically or randomly allocated to intraportal 5-fluorouracil infusion or both). TS and p53 status were determined, blinded to any clinical data, by immunohistochemistry using a validated polyclonal antibody or the DO-7 clone, respectively, and their relationships with overall survival were examined., Results: High TS expression was observed in 58% and overexpression of p53 in 60% of tumours. TS expression correlated with tumour stage, and p53 overexpression, with rectal cancers. There was no evidence that either marker was significantly associated with survival by either univariate (TS hazard ratio (HR) = 0.94, 95% CI 0.76-1.18 and P = 0.6 and p53 HR = 0.98, 95% CI 0.78-1.23 and P = 0.9) or multivariate analyses (TS HR = 0.99, 95% CI 0.79-1.25 and P = 0.9 and p53 HR = 0.98, 95% CI 0.78-1.23 and P = 0.8)., Conclusions: Neither TS nor p53 expression has significant prognostic value in the adjuvant setting of CRC.

Published
2006
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4. Structure-activity relationships in purine-based inhibitor binding to HSP90 isoforms.

Author

Wright L, Barril X, Dymock B, Sheridan L, Surgenor A, Beswick M, Drysdale M, Collier A, Massey A, Davies N, Fink A, Fromont C, Aherne W, Boxall K, Sharp S, Workman P, and Hubbard RE

Subjects
Adenine metabolism, Adenine pharmacology, Anisoles metabolism, Anisoles pharmacology, Binding Sites, Cell Division drug effects, Drug Evaluation, Preclinical, Enzyme Inhibitors metabolism, Enzyme Inhibitors pharmacology, HSP90 Heat-Shock Proteins antagonists & inhibitors, Humans, Ligands, Models, Molecular, Molecular Structure, Protein Isoforms, Protein Structure, Tertiary, Purines metabolism, Purines pharmacology, Structure-Activity Relationship, Adenine analogs & derivatives, Adenine chemistry, Adenosine Triphosphatases antagonists & inhibitors, Anisoles chemistry, Enzyme Inhibitors chemistry, HSP90 Heat-Shock Proteins chemistry, Purines chemistry
Abstract

Inhibition of the ATPase activity of the chaperone protein HSP90 is a potential strategy for treatment of cancers. We have determined structures of the HSP90alpha N-terminal domain complexed with the purine-based inhibitor, PU3, and analogs with enhanced potency both in enzyme and cell-based assays. The compounds induce upregulation of HSP70 and downregulation of the known HSP90 client proteins Raf-1, CDK4, and ErbB2, confirming that the molecules inhibit cell growth by a mechanism dependent on HSP90 inhibition. We have also determined the first structure of the N-terminal domain of HSP90beta, complexed with PU3. The structures allow a detailed rationale to be developed for the observed affinity of the PU3 class of compounds for HSP90 and also provide a structural framework for design of compounds with improved binding affinity and drug-like properties.

Published
2004
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5. High-throughput screening assay for inhibitors of heat-shock protein 90 ATPase activity.

Author

Rowlands MG, Newbatt YM, Prodromou C, Pearl LH, Workman P, and Aherne W

Subjects
Adenosine Triphosphatases metabolism, Colorimetry, Enzyme Inhibitors pharmacology, Fungal Proteins isolation & purification, Fungal Proteins metabolism, HSP90 Heat-Shock Proteins isolation & purification, HSP90 Heat-Shock Proteins metabolism, Phosphates analysis, Adenosine Triphosphatases antagonists & inhibitors, Drug Screening Assays, Antitumor methods, HSP90 Heat-Shock Proteins antagonists & inhibitors
Abstract

The molecular chaperone heat-shock protein 90 (HSP90) plays a key role in the cell by stabilizing a number of client proteins, many of which are oncogenic. The intrinsic ATPase activity of HSP90 is essential to this activity. HSP90 is a new cancer drug target as inhibition results in simultaneous disruption of several key signaling pathways, leading to a combinatorial approach to the treatment of malignancy. Inhibitors of HSP90 ATPase activity including the benzoquinone ansamycins, geldanamycin and 17-allylamino-17-demethoxygeldanamycin, and radicicol have been described. A high-throughput screen has been developed to identify small-molecule inhibitors that could be developed as therapeutic agents with improved pharmacological properties. A colorimetric assay for inorganic phosphate, based on the formation of a phosphomolybdate complex and subsequent reaction with malachite green, was used to measure the ATPase activity of yeast HSP90. The Km for ATP determined in the assay was 510+/-70 microM. The known HSP90 inhibitors geldanamycin and radicicol gave IC(50) values of 4.8 and 0.9 microM respectively, which compare with values found using the conventional coupled-enzyme assay. The assay was robust and reproducible (2-8% CV) and used to screen a compound collection of approximately 56,000 compounds in 384-well format with Z' factors between 0.6 and 0.8.

Published
2004
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6. High-throughput screening for the identification of small-molecule inhibitors of retinoblastoma protein phosphorylation in cells.

Author

Barrie SE, Eno-Amooquaye E, Hardcastle A, Platt G, Richards J, Bedford D, Workman P, Aherne W, Mittnacht S, and Garrett MD

Subjects
Animals, Antibodies, Monoclonal metabolism, Cell Line, Tumor, Cell Membrane chemistry, Drug Evaluation, Preclinical methods, Female, Humans, Mice, Phosphorylation, Purines pharmacology, Retinoblastoma Protein antagonists & inhibitors, Roscovitine, Fluoroimmunoassay methods, Retinoblastoma Protein metabolism
Abstract

The tumor suppressor protein, pRb, regulates progression through the G1 phase of the cell cycle by its ability to bind to and regulate the activity of a variety of transcription factors. This function of pRb is disabled through its phosphorylation by the cyclin-dependent kinase (CDK) family of serine/threonine kinases. In many human cancers, genetic alteration such as loss of CDK inhibitor function and deregulated G1 cyclin expression leads to inappropriate phosphorylation and hence inactivation of this tumor suppressor. Identification of cell-permeable small molecules that block pRb phosphorylation in these tumors could therefore lead to development of an effective anticancer treatment. As a result, we have developed a high-throughput assay to detect changes in the level of pRb phosphorylation in cells. Signal detection is by a time-resolved fluorescence-based cellular immunosorbant assay on a fixed monolayer of cells. This comprises a mouse monoclonal antibody that recognizes the phosphorylated form of serine 608 on pRb, a known site of CDK phosphorylation, and a Europium-labeled secondary antibody for signal detection. The assay is reproducible and amenable to automation and has been used to screen 2000 compounds in a search for cell-permeable small molecules that will block pRb phosphorylation.

Published
2003
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8. Some morphometric methods for the central nervous system.

Author

Aherne W

Subjects
Brain ultrastructure, Cell Count, Humans, Methods, Microscopy, Electron, Purkinje Cells ultrastructure, Brain anatomy & histology, Histological Techniques, Neurons ultrastructure
Abstract

It is the quantitative study of the central nervous system to enumerate neurone populations. Since neurones are generally arranged in non-random patterns the conventional method of counting with a square lattice graticule in the ocular of the microscope is severely restricted. Appropriately tailored methods of (a) counting, or (b) estimating the density of a neurone population must therefore be used. Four types of neuronal distribution pattern are discussed and morphometric methods adapted to them are presented, as follows: (1) Where the whole population is circumscribed, as in the anterior horn motor neurones of the cord, direct counting is feasible. Only those cells whose nucleoli are visible should be included; this diminishes the bias in favour of large cells, and if one corrects for the fact that larger neurones have larger nucleoli the bias can be eliminated completely. (2) Where neurones are situated on an "interface", as Purkinje cells are, the length of its profile (in this instance the boundary between the molecular and granular zones) is estimated by superimposing parallel lines on the microscopical image and counting intersections as these lines cross the interface. The number of Purkinje cells in each particular field is counted at the same time. A "linear dinsity" (PL) is then calculated from the formula pl = 2n/pid where n is the quotient of (a) the number of cells counted along (b) an estimated length of profile, and d is the distance between the parallel lines of the graticule. For comparative studies between cerebella of different sizes a correction factor is easily introduced. Those who prefer to work on photomicrographs can use a mapping wheel to measure a length of profile and then proceed as before. (3) Where neurones are organised in a curving band, as in the dentate nucleus, another form of cell density can be established. The microscope is focused on a neurone at random, and the distance from this cell to its nearest neighbour is measured, preferably by means of a screw-micrometer eyepiece. The mean value r of a number of such measurements is substituted in a formula which gives the "areal density" of the neurone population: pa = 1/4r2. This method can be applied to photomicrographs by using a pair of dividers and/or an accurate rule to measure the set of r values. (4) In large collections of neurones, e.g., in the thalamus, three methods are available: (a) the nearest neighbour method; (b) a conventional squared graticule count, and (c) a count of cells intersected by a line probe as in Haug's (1972) technique (fig. 5), or a modified form of Strong's (1966) transect method.

Published
1975
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12. The vanishing testis.

Author

Abeyaratne MR, Aherne WA, and Scott JE

Subjects
Adolescent, Child, Cryptorchidism surgery, Humans, Male, Vas Deferens abnormalities, Testis abnormalities
Published
1969
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13. Fibrocartilage in the heart.

Author

Balogh K, Ferris JA, and Aherne WA

Subjects
Death, Sudden, Humans, Infant, Cartilage, Heart Conduction System pathology, Heart Defects, Congenital pathology
Published
1971
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