ABSTRACT
Thermoluminescence and optically stimulated luminescence properties of phosphate glasses doped with BaO and Li(2)O at various concentrations were studied. Lithium-doped glasses show a broad TL peak in the 200-300°C region with poor dosimetric characteristics. Barium-doped glasses feature at least two TL peaks, approximately at 200 and 400°C, which were attributed to Ba(2+) ions. They also produce a fast-decaying OSL signal correlated with the lower-temperature TL peak. Responses of both TL emissions to radiation doses up to 100 Gy are linear (R² >0.99). Due to its encouraging characteristics such as acceptable batch homogeneity, good measurement reproducibility and weak signal fading, the P2O5-xBaO glass can be considered as a candidate material for dosimetry in the high-dose range (>10 Gy).
Subject(s)
Glass/chemistry , Thermoluminescent Dosimetry/methods , Luminescence , Materials Testing , Thermoluminescent Dosimetry/instrumentationABSTRACT
The analysis of phenotypic change resulting from gene disruption following homologous recombination provides a powerful technique for the study of gene function. This technique has so far been difficult to apply to plants because the frequency of gene disruption following transformation with constructs containing DNA homologous to genomic sequences is low (0.01 to 0.1%). It has recently been shown that high rates of gene disruption (up to 90%) can be achieved in the moss Physcomitrella patens using genomic sequences of unknown function. We have used this system to examine the specificity of gene disruption in Physcomitrella using a member of the Cab multigene family. We have employed the previously characterised Cab gene ZLAB1 and have isolated segments of 13 other closely related members of the Cab gene family. In the 199-bp stretch sequenced, the 13 new members of the Cab family show an average of 8.5% divergence from the DNA sequence of ZLAB1. We observed 304 silent substitutions and 16 substitutions that lead to a change in the amino acid sequence of the protein. We cloned 1029 bp of the coding region of ZLAB1 (including 177 of the 199 bp with high homology to the 13 new Cab genes) into a vector containing a selectable hygromycin resistance marker, and used this construct to transform P. patens. In three of nine stable transformants tested, the construct had inserted in, and disrupted, the ZLAB1 gene. There was no discernible phenotype associated with the disruption. We have therefore shown that gene disruption is reproducible in P. patens and that the requirement for sequence homology appears to be stringent, therefore allowing the role of individual members of a gene family to be analysed in land plants for the first time.
