-
Something wrong with this record ?
Detection of summer truffle (Tuber aestivum Vittad.) in ectomycorrhizae and in soil using specific primers
M. Gryndler, H. Hršelová, L. Soukupová, E. Streiblová, S. Valda, J. Borovička, H. Gryndlerová, J. Gažo, M. Miko,
Language English Country England, Great Britain
Document type Evaluation Study, Journal Article, Research Support, Non-U.S. Gov't
NLK
ProQuest Central
from 1996-01-01 to 2012-12-31
Medline Complete (EBSCOhost)
from 2006-01-01 to 2014-12-15
Health & Medicine (ProQuest)
from 1996-01-01 to 2012-12-31
Wiley Online Library (archiv)
from 1997-01-01 to 2012-12-31
Public Health Database (ProQuest)
from 1996-01-01 to 2012-12-31
- MeSH
- Ascomycota classification genetics isolation & purification MeSH
- DNA Primers genetics MeSH
- Molecular Sequence Data MeSH
- Mycorrhizae classification genetics isolation & purification MeSH
- Polymerase Chain Reaction instrumentation methods MeSH
- Soil Microbiology MeSH
- Publication type
- Journal Article MeSH
- Evaluation Study MeSH
- Research Support, Non-U.S. Gov't MeSH
Tuber aestivum is becoming an important commodity of great economical value in some European countries. At the same time, it is a highly protected organism in other countries, where it needs careful treatment. A reliable method of detection in roots and soil is thus needed for assessment of geographic distribution, ecological studies and inoculation efficiency testing in man-made experiments. A PCR-based method of detection of T. aestivum using specific primers was therefore developed. A pair of PCR primers Tu1sekvF/Tu2sekvR selective for T. aestivum and some genotypes of Tuber mesentericum was designed on the basis of the known internal transcribed spacer T. aestivum sequences. TaiI restriction cleavage was then used to distinguish the two species. The selectivity of the designed primer pair was evaluated using DNA extracted from specimens of a further 13 Tuber spp. Subsequently, the selectivity and robustness to false-positive results with nontarget DNA of the designed primers was compared with two other primer pairs (UncI/UncII and BTAE-F/BTAEMB-R). The occurrence of T. aestivum in soil and ectomycorrhizae collected in its native habitat has been successfully detected using the designed primers and nested PCR. The method is reliable and thus suitable for detection of T. aestivum in the field.
References provided by Crossref.org
- 000
- 00000naa a2200000 a 4500
- 001
- bmc12027754
- 003
- CZ-PrNML
- 005
- 20121207102355.0
- 007
- ta
- 008
- 120817e20110308enk f 000 0#eng||
- 009
- AR
- 024 7_
- $a 10.1111/j.1574-6968.2011.02243.x $2 doi
- 035 __
- $a (PubMed)21385201
- 040 __
- $a ABA008 $b cze $d ABA008 $e AACR2
- 041 0_
- $a eng
- 044 __
- $a enk
- 100 1_
- $a Gryndler, Milan $u Institute of Microbiology, ASCR, Prague, Czech Republic. gryndler@biomed.cas.cz
- 245 10
- $a Detection of summer truffle (Tuber aestivum Vittad.) in ectomycorrhizae and in soil using specific primers / $c M. Gryndler, H. Hršelová, L. Soukupová, E. Streiblová, S. Valda, J. Borovička, H. Gryndlerová, J. Gažo, M. Miko,
- 520 9_
- $a Tuber aestivum is becoming an important commodity of great economical value in some European countries. At the same time, it is a highly protected organism in other countries, where it needs careful treatment. A reliable method of detection in roots and soil is thus needed for assessment of geographic distribution, ecological studies and inoculation efficiency testing in man-made experiments. A PCR-based method of detection of T. aestivum using specific primers was therefore developed. A pair of PCR primers Tu1sekvF/Tu2sekvR selective for T. aestivum and some genotypes of Tuber mesentericum was designed on the basis of the known internal transcribed spacer T. aestivum sequences. TaiI restriction cleavage was then used to distinguish the two species. The selectivity of the designed primer pair was evaluated using DNA extracted from specimens of a further 13 Tuber spp. Subsequently, the selectivity and robustness to false-positive results with nontarget DNA of the designed primers was compared with two other primer pairs (UncI/UncII and BTAE-F/BTAEMB-R). The occurrence of T. aestivum in soil and ectomycorrhizae collected in its native habitat has been successfully detected using the designed primers and nested PCR. The method is reliable and thus suitable for detection of T. aestivum in the field.
- 650 _2
- $a Ascomycota $x klasifikace $x genetika $x izolace a purifikace $7 D001203
- 650 _2
- $a DNA primery $x genetika $7 D017931
- 650 _2
- $a molekulární sekvence - údaje $7 D008969
- 650 _2
- $a mykorhiza $x klasifikace $x genetika $x izolace a purifikace $7 D038821
- 650 _2
- $a polymerázová řetězová reakce $x přístrojové vybavení $x metody $7 D016133
- 650 _2
- $a půdní mikrobiologie $7 D012988
- 655 _2
- $a hodnotící studie $7 D023362
- 655 _2
- $a časopisecké články $7 D016428
- 655 _2
- $a práce podpořená grantem $7 D013485
- 700 1_
- $a Hršelová, Hana
- 700 1_
- $a Soukupová, Lucie
- 700 1_
- $a Streiblová, Eva
- 700 1_
- $a Valda, Slavomír
- 700 1_
- $a Borovička, Jan
- 700 1_
- $a Gryndlerová, Hana
- 700 1_
- $a Gažo, Ján
- 700 1_
- $a Miko, Marián
- 773 0_
- $w MED00001792 $t FEMS microbiology letters $x 1574-6968 $g Roč. 318, č. 1 (20110308), s. 84-91
- 856 41
- $u https://pubmed.ncbi.nlm.nih.gov/21385201 $y Pubmed
- 910 __
- $a ABA008 $b sig $c sign $y m
- 990 __
- $a 20120817 $b ABA008
- 991 __
- $a 20121207102429 $b ABA008
- 999 __
- $a ok $b bmc $g 949796 $s 785100
- BAS __
- $a 3
- BAS __
- $a PreBMC
- BMC __
- $a 2011 $b 318 $c 1 $d 84-91 $e 20110308 $i 1574-6968 $m FEMS microbiology letters $n FEMS Microbiol Lett $x MED00001792
- LZP __
- $a Pubmed-20120817/11/03
