55 research outputs found
Radiocarbon dating of methane and carbon dioxide evaded from a temperate peatland stream
Streams draining peatlands export large quantities of carbon in different chemical forms and
are an important part of the carbon cycle. Radiocarbon (14C) analysis/dating provides unique
information on the source and rate that carbon is cycled through ecosystems, as has recently
been demonstrated at the air-water interface through analysis of carbon dioxide (CO2) lost
from peatland streams by evasion (degassing). Peatland streams also have the potential to
release large amounts of methane (CH4) and, though 14C analysis of CH4 emitted by ebullition
(bubbling) has been previously reported, diffusive emissions have not. We describe methods
that enable the 14C analysis of CH4 evaded from peatland streams. Using these methods, we
investigated the 14C age and stable carbon isotope composition of both CH4 and CO2 evaded
from a small peatland stream draining a temperate raised mire. Methane was aged between
1617-1987 years BP, and was much older than CO2 which had an age range of 303-521 years
BP. Isotope mass balance modelling of the results indicated that the CO2 and CH4 evaded
from the stream were derived from different source areas, with most evaded CO2 originating
from younger layers located nearer the peat surface compared to CH4. The study demonstrates
the insight that can be gained into peatland carbon cycling from a methodological
development which enables dual isotope (14C and 13C) analysis of both CH4 and CO2 collected
at the same time and in the same way
Protein quality control: the who’s who, the where’s and therapeutic escapes
In cells the quality of newly synthesized proteins is monitored in regard to proper folding and correct assembly in the early secretory pathway, the cytosol and the nucleoplasm. Proteins recognized as non-native in the ER will be removed and degraded by a process termed ERAD. ERAD of aberrant proteins is accompanied by various changes of cellular organelles and results in protein folding diseases. This review focuses on how the immunocytochemical labeling and electron microscopic analyses have helped to disclose the in situ subcellular distribution pattern of some of the key machinery proteins of the cellular protein quality control, the organelle changes due to the presence of misfolded proteins, and the efficiency of synthetic chaperones to rescue disease-causing trafficking defects of aberrant proteins
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