Diversity of denitrifying microflora and ability to reduce N sub(2)O in two soils
The ozone-depleting gas N sub(2)O is an intermediate in denitrification, the biological reduction of NO sub(3) super(-) to the gaseous products N sub(2)O and N sub(2) gas. The molar ratio of N sub(2)O produced (N sub(2)O/N sub(2)O+N sub(2)) varies temporally and spatially, and in some soils N sub(2)...
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| Veröffentlicht in: | Biology and fertility of soils 1998-11, Vol.28 (1), p.19-26 |
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| creator | Cheneby, D Hartmann, A Henault, C Topp, E Germon, J C |
| description | The ozone-depleting gas N sub(2)O is an intermediate in denitrification, the biological reduction of NO sub(3) super(-) to the gaseous products N sub(2)O and N sub(2) gas. The molar ratio of N sub(2)O produced (N sub(2)O/N sub(2)O+N sub(2)) varies temporally and spatially, and in some soils N sub(2)O may be the dominant end product of denitrification. The fraction of NO sub(3) super(-)-N emitted as N sub(2)O may be due at least in part to the abundance and activity of denitrifying bacteria which possess N sub(2)O reductase. In this study, we enumerated NO sub(3) super(-)-reducing and denitrifying bacteria, and compared and contrasted collections of denitrifying bacteria isolated from two agricultural soils, one (Auxonne, soil A) with N sub(2)O as the dominant product of denitrification, the other (Chalons, soil C) with N sub(2) gas as the dominant product. Isolates were tested for the ability to reduce N sub(2)O, and the presence of the N sub(2)O reductase (nosZ)-like gene was evaluated by polymerase chain reaction (PCR) using specific primers coupled with DNA hybridization using a specific probe. The diversity and phylogenetic relationships of members of the collections were established by PCR/restriction fragment length polymorphism of 16s rDNA. The two soils had similar numbers of bacteria which used NO sub(3) super(-) as a terminal electron acceptor anaerobically. However, the soil A had many more denitrifiers which reduced NO sub(3) super(-) to gaseous products (N sub(2)O or N sub(2)) than did soil C. Collections of 258 and 281 bacteria able to grow anaerobically in the presence of NO sub(3) super(-) were isolated from soil A and soil C, respectively. These two collections contained 66 and 12 denitrifying isolates, respectively, the others reducing NO sub(3) super(-) only as far as NO sub(2) super(-). The presence of nosZ sequences was generally a poor predictor of N sub(2)O reducing ability: there was agreement between the occurrence of nosZ sequences and the N sub(2)O reducing ability for only 42% of the isolates; 35% of the isolates (found exclusively in soil A) without detectable nosZ sequences reduced N sub(2)O whereas 21% of the isolates carrying nosZ sequences did not reduce this gas under our assay conditions. Twenty-eight different 16S rDNA restriction patterns (using two restriction endonucleases) were distinguished among the 78 denitrifying isolates. Two types of patterns appeared to be common to both soils. Twenty-three and three types of |
| doi_str_mv | 10.1007/s003740050458 |
| format | Article |
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The molar ratio of N sub(2)O produced (N sub(2)O/N sub(2)O+N sub(2)) varies temporally and spatially, and in some soils N sub(2)O may be the dominant end product of denitrification. The fraction of NO sub(3) super(-)-N emitted as N sub(2)O may be due at least in part to the abundance and activity of denitrifying bacteria which possess N sub(2)O reductase. In this study, we enumerated NO sub(3) super(-)-reducing and denitrifying bacteria, and compared and contrasted collections of denitrifying bacteria isolated from two agricultural soils, one (Auxonne, soil A) with N sub(2)O as the dominant product of denitrification, the other (Chalons, soil C) with N sub(2) gas as the dominant product. Isolates were tested for the ability to reduce N sub(2)O, and the presence of the N sub(2)O reductase (nosZ)-like gene was evaluated by polymerase chain reaction (PCR) using specific primers coupled with DNA hybridization using a specific probe. The diversity and phylogenetic relationships of members of the collections were established by PCR/restriction fragment length polymorphism of 16s rDNA. The two soils had similar numbers of bacteria which used NO sub(3) super(-) as a terminal electron acceptor anaerobically. However, the soil A had many more denitrifiers which reduced NO sub(3) super(-) to gaseous products (N sub(2)O or N sub(2)) than did soil C. Collections of 258 and 281 bacteria able to grow anaerobically in the presence of NO sub(3) super(-) were isolated from soil A and soil C, respectively. These two collections contained 66 and 12 denitrifying isolates, respectively, the others reducing NO sub(3) super(-) only as far as NO sub(2) super(-). The presence of nosZ sequences was generally a poor predictor of N sub(2)O reducing ability: there was agreement between the occurrence of nosZ sequences and the N sub(2)O reducing ability for only 42% of the isolates; 35% of the isolates (found exclusively in soil A) without detectable nosZ sequences reduced N sub(2)O whereas 21% of the isolates carrying nosZ sequences did not reduce this gas under our assay conditions. Twenty-eight different 16S rDNA restriction patterns (using two restriction endonucleases) were distinguished among the 78 denitrifying isolates. Two types of patterns appeared to be common to both soils. Twenty-three and three types of patterns were found exclusively among bacteria isolated from soils A and C, respectively. The specific composition of denitrifying communities appeared to be different between the two soils studied. 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The molar ratio of N sub(2)O produced (N sub(2)O/N sub(2)O+N sub(2)) varies temporally and spatially, and in some soils N sub(2)O may be the dominant end product of denitrification. The fraction of NO sub(3) super(-)-N emitted as N sub(2)O may be due at least in part to the abundance and activity of denitrifying bacteria which possess N sub(2)O reductase. In this study, we enumerated NO sub(3) super(-)-reducing and denitrifying bacteria, and compared and contrasted collections of denitrifying bacteria isolated from two agricultural soils, one (Auxonne, soil A) with N sub(2)O as the dominant product of denitrification, the other (Chalons, soil C) with N sub(2) gas as the dominant product. Isolates were tested for the ability to reduce N sub(2)O, and the presence of the N sub(2)O reductase (nosZ)-like gene was evaluated by polymerase chain reaction (PCR) using specific primers coupled with DNA hybridization using a specific probe. The diversity and phylogenetic relationships of members of the collections were established by PCR/restriction fragment length polymorphism of 16s rDNA. The two soils had similar numbers of bacteria which used NO sub(3) super(-) as a terminal electron acceptor anaerobically. However, the soil A had many more denitrifiers which reduced NO sub(3) super(-) to gaseous products (N sub(2)O or N sub(2)) than did soil C. Collections of 258 and 281 bacteria able to grow anaerobically in the presence of NO sub(3) super(-) were isolated from soil A and soil C, respectively. These two collections contained 66 and 12 denitrifying isolates, respectively, the others reducing NO sub(3) super(-) only as far as NO sub(2) super(-). The presence of nosZ sequences was generally a poor predictor of N sub(2)O reducing ability: there was agreement between the occurrence of nosZ sequences and the N sub(2)O reducing ability for only 42% of the isolates; 35% of the isolates (found exclusively in soil A) without detectable nosZ sequences reduced N sub(2)O whereas 21% of the isolates carrying nosZ sequences did not reduce this gas under our assay conditions. Twenty-eight different 16S rDNA restriction patterns (using two restriction endonucleases) were distinguished among the 78 denitrifying isolates. Two types of patterns appeared to be common to both soils. Twenty-three and three types of patterns were found exclusively among bacteria isolated from soils A and C, respectively. The specific composition of denitrifying communities appeared to be different between the two soils studied. 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The molar ratio of N sub(2)O produced (N sub(2)O/N sub(2)O+N sub(2)) varies temporally and spatially, and in some soils N sub(2)O may be the dominant end product of denitrification. The fraction of NO sub(3) super(-)-N emitted as N sub(2)O may be due at least in part to the abundance and activity of denitrifying bacteria which possess N sub(2)O reductase. In this study, we enumerated NO sub(3) super(-)-reducing and denitrifying bacteria, and compared and contrasted collections of denitrifying bacteria isolated from two agricultural soils, one (Auxonne, soil A) with N sub(2)O as the dominant product of denitrification, the other (Chalons, soil C) with N sub(2) gas as the dominant product. Isolates were tested for the ability to reduce N sub(2)O, and the presence of the N sub(2)O reductase (nosZ)-like gene was evaluated by polymerase chain reaction (PCR) using specific primers coupled with DNA hybridization using a specific probe. The diversity and phylogenetic relationships of members of the collections were established by PCR/restriction fragment length polymorphism of 16s rDNA. The two soils had similar numbers of bacteria which used NO sub(3) super(-) as a terminal electron acceptor anaerobically. However, the soil A had many more denitrifiers which reduced NO sub(3) super(-) to gaseous products (N sub(2)O or N sub(2)) than did soil C. Collections of 258 and 281 bacteria able to grow anaerobically in the presence of NO sub(3) super(-) were isolated from soil A and soil C, respectively. These two collections contained 66 and 12 denitrifying isolates, respectively, the others reducing NO sub(3) super(-) only as far as NO sub(2) super(-). The presence of nosZ sequences was generally a poor predictor of N sub(2)O reducing ability: there was agreement between the occurrence of nosZ sequences and the N sub(2)O reducing ability for only 42% of the isolates; 35% of the isolates (found exclusively in soil A) without detectable nosZ sequences reduced N sub(2)O whereas 21% of the isolates carrying nosZ sequences did not reduce this gas under our assay conditions. Twenty-eight different 16S rDNA restriction patterns (using two restriction endonucleases) were distinguished among the 78 denitrifying isolates. Two types of patterns appeared to be common to both soils. Twenty-three and three types of patterns were found exclusively among bacteria isolated from soils A and C, respectively. The specific composition of denitrifying communities appeared to be different between the two soils studied. This may partly explain the differences in the behaviour of the soils concerning N sub(2)O reduction during denitrification.</abstract><doi>10.1007/s003740050458</doi></addata></record> |
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| title | Diversity of denitrifying microflora and ability to reduce N sub(2)O in two soils |
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