Deletion of high-molecular-weight glutenin subunits in wheat significantly reduced dough strength and bread-baking quality

Yingjun Zhang; Mengyun Hu; Qian Liu; Lijing Sun; Xiyong Chen; Liangjie Lv; Yuping Liu; Xu Jia; Hui Li

doi:10.1186/s12870-018-1530-z

Deletion of high-molecular-weight glutenin subunits in wheat significantly reduced dough strength and bread-baking quality

BMC Plant Biol. 2018 Dec 3;18(1):319. doi: 10.1186/s12870-018-1530-z.

Authors

Yingjun Zhang¹, Mengyun Hu¹, Qian Liu¹, Lijing Sun¹, Xiyong Chen¹, Liangjie Lv¹, Yuping Liu¹, Xu Jia², Hui Li³

Affiliations

¹ Institute of Cereal and Oil Crops, Hebei Academy of Agriculture and Forestry Sciences, 162 Hengshan Street, Shijiazhuang, 050035, China.
² Institute of Genetics and Developmental Biology, Chinese Academy of Sciences, 1 Beichenxi Road, Beijing, 100101, China.
³ Institute of Cereal and Oil Crops, Hebei Academy of Agriculture and Forestry Sciences, 162 Hengshan Street, Shijiazhuang, 050035, China. zwslihui@163.com.

Abstract

Background: High-molecular-weight glutenin subunits (HMW-GS) play important roles in the elasticity of dough made from wheat. The HMW-GS null line is useful for studying the contribution of HMW-GS to the end-use quality of wheat.

Methods: In a previous work, we cloned the Glu-1E^bx gene from Thinopyrum bessarabicum and introduced it into the wheat cultivar, Bobwhite. In addition to lines expressing the Glu-1E^bx gene, we also obtained a transgenic line (LH-11) with all the HMW-GS genes silenced. The HMW-GS deletion was stably inherited as a dominant and conformed to Mendel's laws. Expression levels of HMW-GS were determined by RT-PCR and epigenetic changes in methylation patterns and small RNAs were analyzed. Glutenins and gliadins were separated and quantitated by reversed-phase ultra-performance liquid chromatography. Measurement of glutenin macropolymer, and analysis of agronomic traits and end-use quality were also performed.

Results: DNA methylation and the presence of small double-stranded RNA may be the causes of post-transcriptional gene silencing in LH-11. The accumulation rate and final content of glutenin macropolymer (GMP) in LH-11 were significantly lower than in wild-type (WT) Bobwhite. The total protein content was not significantly affected as the total gliadin content increased in LH-11 compared to WT. Deletion of HMW-GS also changed the content of different gliadin fractions. The ratio of ω-gliadin increased, whereas α/β- and γ-gliadins declined in LH-11. The wet gluten content, sedimentation value, development time and stability time of LH-11 were remarkably lower than that of Bobwhite. Bread cannot be made using the flour of LH-11.

Conclusions: Post-transcriptional gene silencing through epigenetic changes and RNA inhibition appear to be the causes for the gene expression deficiency in the transgenic line LH-11. The silencing of HMW-GW in LH-11 significantly reduced the dough properties, GMP content, wet gluten content, sedimentation value, development time and stability time of flour made from this wheat cultivar. The HMW-GS null line may provide a potential material for biscuit-making because of its low dough strength.

Keywords: Common wheat; Dough quality; Gliadin content; Glutenin macropolymer; High-molecular-weight glutenin subunits; Post-transcriptional gene silencing.

MeSH terms

Bread* / standards
Cooking
DNA Methylation
Flour
Glutens / genetics
Glutens / metabolism*
Plant Proteins / genetics
Plant Proteins / metabolism*
Plants, Genetically Modified
RNA Interference
Seeds / growth & development
Seeds / metabolism
Triticum / genetics
Triticum / metabolism*

Substances

Plant Proteins
Glutens
glutenin

Abstract

MeSH terms

Substances

Grants and funding