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Experimental taphonomy: silicification of plants in Yellowstone hot-spring environments

Published online by Cambridge University Press:  26 July 2007

Alan Channing
Affiliation:
School of Earth, Ocean and Planetary Sciences, Cardiff University, Cardiff CF10 3YE, UK.
Dianne Edwards
Affiliation:
School of Earth, Ocean and Planetary Sciences, Cardiff University, Cardiff CF10 3YE, UK.

Abstract

During experiments conducted within the vent pool of Medusa Geyser, Norris Geyser Basin, Yellowstone National Park, USA, amorphous opaline silica (opal-A) was deposited on/within plant tissues within 30 days of immersion. Initially, deposition created inter/intra-cellular films which lined cell walls plus intercellular colloid suspensions (sols) of opal-A nano/microspheres. By 330 days, opal-A deposition created a robust external and internal matrix that stabilised tissues against collapse and replicated plant structure. Opal-A films increased to micron-order thicknesses and intracellular sols were created. Systematic variation of opal-A fabric between tissues comprising living/dead cells at the time of deposition indicate that cell function, architecture and shape influence fabric development. Heterogeneity of opal-A fabric within adjacent cells of similar structure/function indicates spatially/temporally fluctuating physicochemical conditions and the presence of intraorganic microenvironments. Early deposition of opal-A films suggests a period of low silica supersaturation and slow opal-A deposition. In contrast, intracellular sols suggest high levels of supersaturation, and rapid opal-A deposition. Shell-like microsphere growth suggests cyclic variation of silica supersaturation, and alternations between rapid and slower opal-A deposition. Microsphere growth to the upper limit of colloidal stability and colloidal crystal structures indicate prolonged sol stability, whilst floc-like microsphere networks indicate localised sol instabi

Type
Research Article
Copyright
Royal Society of Edinburgh 2003

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