Issn 305-9397. Ғылым және білім. 2022. №1-1 (66) issn 2305-9397

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Журнал Наука и образование №3-3(68) 2022

______ ____________Ауыл шаруашылығы ғылымдары
174
70-90V for 40 minutes.
a) 1 – sample 81(2); 2 – sample 82-2(1); 3 – sample
82-2; 4 – sample 82-2(2); 5 – sample 82-2(2);
6 – sample 94-1; 7 – sample 95-2; 8 - sample 96;
9 - sample 97; M – 1 Kb Plus DNA Ladder molecular
weight marker.
b)1 – sample 1; 2 – sample 2; 3 – sample 5; 4 – sample
7; 5 – sample 8; 6 – sample 9; 7 – sample 12;
8 – sample 14; 9 - sample 15; M – 1 Kb Plus DNA
Ladder molecular weight marker.
Figure 1 – Electrophoregram: identification of bacterial DNA using the molecular marker 16S (a) and
representatives of the genus Pseudomonas using the molecular marker rpoD (b)
c)1 – sample 1-1; 2 – sample 1-3; 3 – sample 1-5;
4 – sample 1-6; 5 – sample 3-1; 6 – sample 3-2;
7 – sample 3-5; 8 – sample 3-6; 9 – sample 5-2;
M – 1 Kb Plus DNA Ladder molecular weight marker.
d)1 – sample 6-1; 2 – sample 6-2; 3 – sample 6-3;
4 – sample 6-4; 5 – sample 6-5; 6 – sample 6-6;
7 – sample 6-7; 8 – sample 6-8; 9 – sample 6-9;
M – 1 Kb Plus DNA Ladder molecular weight
marker.
Figure 2 – Electrophoregram: identification of bacterial DNA of representatives of the genus
Pseudomonas using the molecular marker gyrB (c) and genus Xanthomonas using the molecular
marker fyuA (lanes 6-9) (d)
e)1 – sample 7-1; 2 – sample 7-2; 3 – sample 7-3;
4 – sample 7-4; 5 – sample 7-5; 6 – sample 7-6; 7 –
sample 7-7; 8 – sample 7-8; 9 – sample 7-9; M – 1 Kb
Plus DNA Ladder molecular weight marker.
f)1 – sample 8-1; 2 – sample 8-2; 3 – sample 8-3;
4 – sample 8-4; 5 – sample 8-5; 6 – sample 8-6;
7 – sample 8-7; 8 – sample 8-8; 9 – sample 8-9;
10 – sample 8-10; 11 – sample 8-11; 12 – sample
8-12; 13 – sample 8-13; 14 – sample 8-14; M – 1 Kb
Plus DNA Ladder molecular weight marker.
Figure 3 – Electrophoregram: identification of bacterial DNA of representatives of the genus
Xanthomonas using the molecular marker rpoD (e) and genus Pseudomonas using the molecular
marker gltA (f)
Thus, ecological and genetic monitoring of pathogens of the most dangerous bacterial diseases
of wheat and other cereal crops was carried out - pathogens of black (Xanthomonas campestris) and
basal (Pseudomonas syringae) bacterioses of wild and agricultural cereal crops. Samples of wild and
agricultural cereal crops were collected in the north of Kazakhstan, and bacterioses infecting cereal

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