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Journal of Integrative Agriculture
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Molecular detection of the powdery mildew resistance genes in winter wheats DH51302 and Shimai 26
QU Yun-feng, WU Pei-pei, HU Jing-huang, CHEN Yong-xing, SHI Zhan-liang, QIU Dan, LI Ya-hui, ZHANG Hong-jun, ZHOU Yang, YANG Li, LIU Hong-wei, ZHU Tong-quan, LIU Zhi-yong, ZHANG Yan-ming, LI Hong-jie
2020, 19 (
4
): 931-940. DOI:
10.1016/S2095-3119(19)62644-4
Abstract
(
122
)
PDF in ScienceDirect
Resistance to powdery mildew is an important trait of interest in many wheat breeding programs. The information on genes conferring resistance to powdery mildew in wheat cultivars is useful in parental selection. Winter wheat breeding line DH51302 derived from Liangxing 99 and cultivar Shimai 26 derived from Jimai 22 showed identical infection patterns against 13 isolates of
Blumeria graminis
f. sp.
tritici
(Bgt) that causes wheat powdery mildew.
DH51302
and Shimai 26 were crossed to a powdery mildew susceptible cultivar Zhongzuo 9504 and the F
2:3
families were used in molecular localization of the resistance genes. Fourteen polymorphic markers, which were linked to
Pm52
from Liangxing 99, were used to establish the genetic linkage maps for the resistance genes
PmDH51302
and
PmSM26
in
DH51302
and Shimai 26, respectively. These genes were placed in the same genetic interval where
Pm52
resides. Analysis of gene-linked molecular markers indicated that
PmDH51302
and
PmSM26
differed from other powdery mildew resistance genes on chromosome arm 2BL, such as
Pm6
,
Pm33
,
Pm51
,
MlZec1
,
MlAB10
, and
Pm64
. Based on the results of reaction patterns to different Bgt isolates and molecular marker localization, together with the pedigree information, DH51302 and Shimai 26 carried the same gene,
Pm52
, which confers their resistance to powdery mildew.
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Genetic progress in stem lodging resistance of the dominant wheat cultivars adapted to Yellow-Huai River Valleys Winter Wheat Zone in China since 1964
ZHANG Hong-jun, LI Teng, LIU Hong-wei, MAI Chun-yan, YU Guang-jun, LI Hui-li, YU Li-qiang, MENG Ling-zhi, JIAN Da-wei, YANG Li, LI Hong-jie, ZHOU Yang
2020, 19 (
2
): 438-448. DOI:
10.1016/S2095-3119(19)62627-4
Abstract
(
144
)
Analysis of genetic progress for lodging-related traits provides important information for further improvement of lodging resistance. Forty winter wheat cultivars widely grown in the Yellow-Huai River Valleys Winter Wheat Zone (YHWZ) of China during the period of 1964–2015 were evaluated for several lodging-related traits in three cropping seasons. Plant height, height at center of gravity, length of the basal second internode, and lodging index decreased significantly in this period, and the average annual genetic gains for these traits were –0.50 cm or –0.62%, –0.27 cm or –0.60%, –0.06 cm or –0.63%, and –0.01 or –0.94%, respectively. Different from other traits, stem strength showed a significant increasing trend with the breeding period, and the annual genetic gains were 0.03 N or 0.05%. Correlation analysis showed that lodging index was positively correlated with plant height, height at center of gravity, and length of the basal second internode, but negatively correlated with stem strength. Meanwhile, significantly positive correlations were observed between plant height, height at center of gravity, and length of the basal first and second internodes. By comparison with the wild types, dwarfing genes had significant effects on all lodging-related traits studied except for length of the basal first internode and stem strength. Principle component analysis demonstrated that plant height and stem strength were the most important factors influencing lodging resistance. Clustering analysis based on the first two principle components further indicated the targets of wheat lodging-resistant breeding have changed from reducing plant height to strengthening stem strength over the breeding periods. This study indicates that the increase of stem strength is vital to improve lodging resistance in this region under the high-yielding condition when plant height is in an optimal range.
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Host status of
Brachypodium distachyon
to the cereal cyst nematode
CHEN Chang-long, LIU Shu-sen, LIU Qian, NIU Jun-hai, LIU Pei, ZHAO Jian-long, LIU Zhi-yong, LI Hong-jie, JIAN Heng
2018, 17 (
2
): 381-388. DOI:
10.1016/S2095-3119(17)61745-3
Abstract
(
726
)
PDF in ScienceDirect
Cereal cyst nematode (
Heterodera avenae
, CCN) distributes worldwide and has caused severe damage to cereal crops, and a model host will greatly aid in the study of this nematode. In this research, we assessed the sensitivity of 25 inbred lines of
Brachypodium distachyon
to
H. avenae
from Beijing, China. All lines of
B. distachyon
were infested by second-stage juveniles (J2s) of
H. avenae
from Daxing District of Beijing population, but only 13 inbred lines reproduced 0.2–3 cysts/plant, showing resistance. The entire root system of the infested
B. distachyon
appeared smaller and the fibrous roots were shorter and less numerous. We found that a dose of 1 000 J2s of
H. avenae
was sufficient for nematode infestation. We showed that Koz-1 of
B. distachyon
could reproduce more cysts than TR2A line. Line Koz-1 also supported the complete life cycles of 5 CCN geographical populations belonging to the Ha1 or Ha3 pathotype group. Our results suggest that
B. distachyon
is a host for CCN.
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Identification of salinity-related genes in
ENO2
mutant (
eno2
–
) of
Arabidopsis thaliana
ZHANG Yong-hua, CHEN Chao, SHI Zi-han, CHENG Hui-mei, BING Jie, MA Xiao-feng, ZHENG Chao-xing, LI Hong-jie, ZHANG Gen-fa
2018, 17 (
01
): 94-110. DOI:
10.1016/S2095-3119(17)61720-9
Abstract
(
668
)
PDF in ScienceDirect
Abiotic stress poses a great threat to plant growth and can lead to huge losses in yield. Gene
enolase2
(
ENO2
) is important in resistance to abiotic stress in various organisms.
ENO2
T-DNA insertion mutant (
eno2
–
) plants of Arabidopsis thaliana showed complete susceptibility to sodium chloride treatment when were analyzed either as whole plants or by measuring root growth during NaCl treatment. Quantitative real-time RT-PCR (RT-qPCR) was performed to investigate the expression profile of
ENO2
in response to NaCl stress in Arabidopsis. The transcript level of
ENO2
was rapidly elevated in 300 mmol L
–1
NaCl treatment. ENO2 also responded to 300 mmol L
–1
NaCl treatment at the protein level. To illuminate the mechanism underlying
ENO2
resistance to salt at the transcriptional level, we studied the wild-type and eno2
–
Arabidopsis
lines that were treated with 300 mmol L
–1
NaCl for 18 h using 454 GS FLX, which resulted in an expressed sequence tag (EST) dataset. A total of 961 up-regulated and 746 down-regulated differentially expressed genes (DEGs) were identified in the pairwise comparison WT-18 h:
eno2
–
-18 h. The DEGs were identified and functionally annotated using the databases of Gene Ontology (GO) and the Kyoto encyclopedia of genes and genomes (KEGG). The identified unigenes were subjected to GO analysis to determine biological, molecular, and cellular functions. The biological process was enriched in a total of 20 GO terms, the cellular component was enriched in 13 GO terms, and the molecular function was enriched in 11 GO terms. Using KEGG mapping, DEGs with pathway annotations contributed to 115 pathways. The top 3 pathways based on a statistical analysis were biosynthesis of the secondary metabolites (KO01110), plant-pathogen interactions (KO04626), and plant hormone signal transduction (KO04075). Based on these results,
ENO2
contributes to increased resistance to abiotic stress. In particular,
ENO2
is involved in some of the metabolic stress response pathways in
Arabidopsis
. Our work also demonstrates that this EST dataset will be a powerful resource for further studies of
ENO2
, such as functional analyses, investigations of biological roles, and molecular breeding. Additionally, 3-phosphoglycerate kinase (PGK), 3-phosphoglycerate kinase 1 (PGK1), triosephosphate isomerase (TPI), and pyruvate kinase (PK) in glycolysis interactions with
ENO2
were verified using the yeast two-hybrid experiment, and
ENO2
may regulate the expression of
PGK
,
PGK1
,
TPI
, and
PK
. Taken together, the results from this study reflects that
ENO2
gene has an important role in the response to the high salt stress.
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Proteomics Identification of Differentially Expressed Leaf Proteins in Response to Setosphaeria turcica Infection in Resistant Maize
ZHANG Xiao-li, SI Bing-wen, FAN Cheng-ming, LI Hong-jie , WANG Xiao-ming
2014, 13 (
4
): 789-803. DOI:
10.1016/S2095-3119(13)60513-4
Abstract
(
2221
)
PDF in ScienceDirect
Northern corn leaf blight (NCLB), caused by the heterothallic ascomycete fungus Setosphaeria turcica, is a destructive foliar disease of maize and represents a serious threat to maize production worldwide. A comparative proteomic study was conducted to explore the molecular mechanisms underlying the defense responses of the maize resistant line A619 Ht2 to S. turcica race 13. Leaf proteins were extracted from mock and S. turcica-infected leaves after inoculated for 72 h and analyzed for differentially expressed proteins using two-dimensional electrophoresis and mass spectrometry identification. 137 proteins showed reproducible differences in abundance by more than 2-fold at least, including 50 up-regulated proteins and 87 down-regulated proteins. 48 protein spots were successfully identified by MS analysis, which included 10 unique, 6 up-regulated, 20 down-regulated and 12 disappeared protein spots. These identified proteins were classified into 9 functional groups and involved in multiple functions, particularly in energy metabolism (46%), protein destination and storage (12%), and disease defense (18%). Some defense-related proteins were upregulated such as β-glucosidase, SOD, polyamines oxidase, HSC 70 and PPIases; while the expressions of photosynthesis- and metabolism-related proteins were down-regulated, by inoculation with S. turcica. The results indicated that a complex regulatory network was functioned in interaction between the resistant line A619 Ht2 and S. turcica. The resistance processes of A619 Ht2 mainly resided on directly releasing defense proteins, modulation of primary metabolism, affecting photosyntesis and carbohydrate metabolism.
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