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Dive into the research topics where A. W. McDowall is active.

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Featured researches published by A. W. McDowall.


Journal of Ultrastructure Research | 1984

On the preparation of cryosections for immunocytochemistry.

Gareth Griffiths; A. W. McDowall; Ruth Back; Jacques Dubochet

The key preparation steps in the Tokuyasu thawed frozen section technique for immunocytochemistry, namely freezing, sectioning, thawing, and drying, were studied. A spherical tissue culture cell was used as a model system. The frozen hydrated section technique indicated that glutaraldehyde-fixed, 2.1 M sucrose-infused pellets of cells were routinely vitrified by immersion in liquid nitrogen but water was crystallized when lower sucrose concentrations (0.6-1 M) were used. Quantitative mass measurements showed that the fixed cells are freely permeable to sucrose. The frozen hydrated sections were severely compressed but cell profiles regained their circular appearance upon thawing. The average section thickness of our frozen-hydrated sections was 110 nm: this was reduced to 30-50 nm upon thawing, washing, and air-drying. This change was accompanied by severe drying artifacts. By using the methyl cellulose drying technique, this collapse upon air-drying could be significantly reduced, but not completely prevented, giving an average thickness of 70 nm.


The EMBO Journal | 2004

Cryo-electron microscopy of vitreous sections

Ashraf Al-Amoudi; Jiin-Ju Chang; Amélie Leforestier; A. W. McDowall; Laurée Michel Salamin; Lars Norlén; Karsten Richter; Nathalie Sartori Blanc; Daniel Studer; Jacques Dubochet

Since the beginning of the 1980s, cryo‐electron microscopy of a thin film of vitrified aqueous suspension has made it possible to observe biological particles in their native state, in the absence of the usual artefacts of dehydration and staining. Combined with 3‐d reconstruction, it has become an important tool for structural molecular biology. Larger objects such as cells and tissues cannot generally be squeezed in a thin enough film. Cryo‐electron microscopy of vitreous sections (CEMOVIS) provides then a solution. It requires vitrification of a sizable piece of biological material and cutting it into ultrathin sections, which are observed in the vitrified state. Each of these operations raises serious difficulties that have now been overcome. In general, the native state seen with CEMOVIS is very different from what has been seen before and it is seen in more detail. CEMOVIS will give its full potential when combined with computerized electron tomography for 3‐d reconstruction.


Australian Journal of Chemistry | 2005

Submicron Dispersions of Hexosomes Based on Novel Glycerate Surfactants

Celesta Fong; Irena Krodkiewska; Darrell Wells; Ben J. Boyd; James Booth; Suresh K. Bhargava; A. W. McDowall; Patrick G. Hartley

Glycerate-based surfactants are a new class of swelling amphiphiles which swell to a finite degree with water. Among this class of surfactants, oleyl (cis-octadec-9-enyl) glycerate is very similar in structure to a well characterized mesophase-forming lipid, glyceryl monooleate (GMO). Despite the similar structural characteristics, a subtle change in connectivity of the ester bond substantially alters the binary surfactant-water phase behaviour. Whereas the phase behaviour of GMO is diverse and dominated by cubic phases, the phase behaviour of oleyl glycerate and a terpenoid analogue phytanyl (3,7,11,15-tetramethyl-hexadecane) glycerate is much simplified. Both exhibit an inverse hexagonal phase (H-II), which is stable to dilution with excess water, and an inverse micellar phase (L-II) at ambient temperatures. The inverse hexagonal phases formed by oleyl glycerate and phytanyl glycerate have been characterized using SAXS. Analogous to GMO cubosomes, the inverse hexagonal phase of phytanyl glycerate has been dispersed to form hexagonally facetted particles, termed hexosomes, whose structure has been verified using cryo-TEM.


Nature | 1984

Cryo-electron microscopy of viruses

Marc Adrian; Jacques Dubochet; Jean Lepault; A. W. McDowall


Plant Biotechnology Journal | 2007

Engineering photosynthetic light capture: Impacts on improved solar energy to biomass conversion

Jan H. Mussgnug; Skye R. Thomas-Hall; Jens Rupprecht; Alexander Foo; Viktor Klassen; A. W. McDowall; Peer M. Schenk; Olaf Kruse; Ben Hankamer


Blood | 2006

A global role for EKLF in definitive and primitive erythropoiesis

Denise J. Hodge; Elise Coghill; Janelle R. Keys; Tina L Maguire; B.M. Hartmann; A. W. McDowall; Mitchell J. Weiss; Sean M. Grimmond; Andrew C. Perkins


Journal of Structural Biology | 2007

SwarmPS: rapid, semi-automated single particle selection software.

David Woolford; Geoffery Ericksson; Rosalba Rothnagel; David A. Muller; Michael J. Landsberg; Radosav S. Pantelic; A. W. McDowall; Bernard Pailthorpe; Paul R. Young; Ben Hankamer; Jasmine Banks


Langmuir | 2007

Wormlike Micelles from a Cage Amine Metallosurfactant

George A. Koutsantonis; Gareth L. Nealon; Craig E. Buckley; Mark Paskevicius; Laurent Douce; Jack M. Harrowfield; A. W. McDowall


Journal of Structural Biology | 2006

The discriminative bilateral filter: an enhanced denoising filter for electron microscopy data.

Radosav S. Pantelic; Rosalba Rothnagel; Chang-Yi Huang; David A. Muller; David Woolford; Michael J. Landsberg; A. W. McDowall; Bernard Pailthorpe; Paul R. Young; Jasmine Banks; Ben Hankamer; Geoffery Ericksson


Microscopy and Microanalysis | 2007

Ultrastructure of Photosynthesis in Green Algae Mutants

Alexander Foo; Benjamin Hankamer; Jan H. Mussgnug; Jens Rupprecht; Olaf Kruse; A. W. McDowall

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Jens Rupprecht

University of Queensland

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Ben Hankamer

University of Queensland

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M. Reyes

University of Queensland

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Alexander Foo

University of Queensland

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David Woolford

University of Queensland

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