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1

The post-symptom and pre-leaf fall, post-harvest activities of several commercial fungicides against apple scab (Venturia inaequalis)

100%
Martin P.
Fruit Science Reports
|
1989
|
tom 16
|
nr 1
2

Floral development and embryology in Lomandra longifolia

63%
Ahmad N., Martin P.
Acta Biologica Cracoviensia. Series Botanica. Supplement
|
2005
|
tom 47
|
nr 1
3

14 IWMS - nowe kierunki w obrobce drewna i tworzyw drzewnych

51%
Miklaszewski S., Beer P., Gogolewski P., Martin P.
Przemysł Drzewny
|
2000
|
tom 51
|
nr 06
26-28
4

Early spawning in tench [Tinca tinca [L.]] under controlled environmental conditions

51%
Martin P., San Juan L. D., Alvarino J. M. R.
Polskie Archiwum Hydrobiologii
|
1999
|
tom 46
|
nr 3-4
5
Content available remote

The major protein fraction of mouse milk revisited using proven proteomic tools

39%
Boumahrou N., Andrei S., Miranda G., Henry C., Panthier J. J., Martin P., Bellier S.
Journal of Physiology and Pharmacology. Supplement
|
2009
|
tom 60
|
nr 3
113-118
6

Genotypes of Listeria monocytogenes strains isolated from 2000 to 2002 in Poland

39%
Paciorek J., Jacquet C., Salcedo C., Doumith M., Vazquez J. A., Martin P.
Polish Journal of Microbiology
|
2006
|
tom 55
|
nr 1
Pulsed field gel electrophoresis (PFGE), multiplex PCR and multilocus sequence typing (MLST) methods were used for genotyping study of seventy-three L. monocytogenes isolates collected in Poland between 2000 and 2002 from human, food, environment and a diseased goat. The multiplex PCR, which is an alternative method to classical serotyping, divided the isolates into four PCR groups, IIa (42.5%), IIb (27.4%), IIc (4.1%) and IVb (26%). The isolates displayed 33 distinct PFGE profiles. Twenty eight strains were further characterised by MLST based on sequence analyses of seven housekeeping genes. The combined sequence analyses revealed a total of 10 different allelic profiles from which 3 were not described earlier. It is intended that results obtained in this study will be the first data of a national database of L. monocytogenes genotypes in Poland.
7

Induction of spawning in tench [Tinca tinca [L.]] by LHRH-A or the complementary administration of a dopaminergic antagonist [Domperidone]

39%
San Juan L. D., Martin P., Busto I., Cea R., Alonso M., Alvarino J. M. R.
Polskie Archiwum Hydrobiologii
|
1999
|
tom 46
|
nr 2
8
Content available remote

A cDNA macroarray resource for gene expression profiling in ruminant tissues involved in reproduction and production (milk and beef) traits

27%
Bernard C., Degrelle S., Ollier S., Campion E., Cassar-Malek I., Charpigny G., Dhorne-Pollet S., Hue I., Hocquette J.-F., Le Provost F., Leroux C., Piumi F., Rolland G., Uzbekova S., Zalachas E., Martin P.
Journal of Physiology and Pharmacology. Supplement
|
2005
|
tom 56
|
nr 3
215-224
cDNA arrays have proven to be useful tools to screen gene expression in many animal species including livestock species. A collaborative program was launched to construct a ruminant cDNA collection, representative of three tissues: Muscle, Embryo and Mammary gland, named MEM. This collection gathers clones mainly arising from 3 non-normalised cDNA libraries: a directed bovine muscle library, a 14-day-old bovine embryo library and a goat lactating mammary library. It is made up of 1896 clones (637 muscle, 882 embryo and 377 mammary cDNAs), selected after sequencing and bioinformatic analyses. Amplification products yielded from these clones as well as controls were printed onto Nylon membranes to generate macroarrays. Hybridisation with relevant cDNA targets allowed checking the location of about 50 cDNAs and the specificity of each sub-set of the repertoire. Macroarrays were hybridised with radiolabelled cDNA complex targets from five different tissues (muscle, embryo, mammary gland, adipose tissue and oocyte). Both somatic and germinal complex targets gave valid hybridisation signals with 45 to 80% of the printed probes. This specific cDNA collection now provides a powerful tool for transcriptomic studies with the ultimate objective to better understand physiological and metabolic functions in ruminants. It will be subsequently included into a forthcoming larger collection.
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