Background Pentatricopeptide repeat (PPR) proteins compose a large protein family whose members are involved in both RNA processing in organelles and plant growth. Previous reports have shown that E-subgroup PPR proteins are involved in RNA editing. However, the additional functions and roles of the E-subgroup PPR proteins are unknown. Results In this study, we developed and identified a new maize kernel mutant with arrested embryo and endosperm development, i.e., defective kernel (dek) 55 (dek55). Genetic and molecular evidence suggested that the defective kernels resulted from a mononucleotide alteration (C to T) at + 449 bp within the open reading frame (ORF) of Zm00001d014471 (hereafter referred to as DEK55). DEK55 encodes an E-subgroup PPR protein within the mitochondria. Molecular analyses showed that the editing percentage of 24 RNA editing sites decreased and that of seven RNA editing sites increased in dek55 kernels, the sites of which were distributed across 14 mitochondrial gene transcripts. Moreover, the splicing efficiency of nad1 introns 1 and 4 and nad4 intron 1 significantly decreased in dek55 compared with the wild type (WT). These results indicate that DEK55 plays a crucial role in RNA editing at multiple sites as well as in the splicing of nad1 and nad4 introns. Mutation in the DEK55 gene led to the dysfunction of mitochondrial complex I. Moreover, yeast two-hybrid assays showed that DEK55 interacts with two multiple organellar RNA-editing factors (MORFs), i.e., ZmMORF1 (Zm00001d049043) and ZmMORF8 (Zm00001d048291). Conclusions Our results demonstrated that a mutation in the DEK55 gene affects the mitochondrial function essential for maize kernel development. Our results also provide novel insight into the molecular functions of E-subgroup PPR proteins involved in plant organellar RNA processing.
Steel shelves are widely used in logistics and warehousing, however, steel shelves often occur instability and other accidents in applications. Many of the destruction are instantaneous. [ Therefore, how to timely monitor the deformation of the shelf, especially the deformation of the shelves on the dynamic stress in the moment to ensure the safe of the shelves is very important. This article describes the method of using digital cameras to monitor dynamic and instantaneous deformation of shelf, which has the characteristics that easy to use, high accuracy, rapid reaction, and observing multi-point once, all-weather use, does not affect the normal work.
Background Pentatricopeptide repeat (PPR) proteins is a large protein family, which participate in RNA processing in organelles and plant growth. Previous reports have generally considered E-subgroup PPR proteins as an editing factors for RNA editing. However, the underlying mechanisms and effects of E-subgroup PPR proteins remain to be investigated.Results In this study, we recognized and identified a new maize kernel mutant with arrested embryo and endosperm development, defective kernel 55 (dek55). Genetic and molecular evidences suggest that the defective kernels resulted from a mononucleotide alteration (C to T) at + 449 in the open reading frame (ORF) of Zm00001d014471 (hereafter referred to as DEK55). DEK55 encodes an E-subgroup PPR protein within mitochondria. Molecular analyses suggest that DEK55 plays crucial roles in RNA editing at multiple sites of ribosomal protein S13, ATP synthase subunit1, NADH dehydrogenase-6 (nad6), and nad9 transcripts as well as in splicing of nad1 and nad4. The mutation of DEK55 lead to the dysfunction of mitochondrial complex I.Conclusions Our results demonstrate that the DEK55 mutation is responsible for the dek55 mutant phenotypes, as it affects mitochondrial function that is essential for maize kernel development. This study also provides novel insight into the molecular function of E-subgroup PPR proteins in plant organellar RNA metabolism.
Background: Pentatricopeptide repeat (PPR) proteins compose a large protein family whose members are involved in both RNA processing in organelles and plant growth. Previous reports have shown that E-subgroup PPR proteins are involved in RNA editing. However, the additional functions and roles of the E-subgroup PPR proteins are unknown. Results: In this study, we developed and identified a new maize kernel mutant with arrested embryo and endosperm development, i.e., defective kernel (dek) 55 (dek55). Genetic and molecular evidence suggested that the defective kernels resulted from a mononucleotide alteration (C to T) at +449 bp within the open reading frame (ORF) of Zm00001d014471 (hereafter referred to as DEK55). DEK55 encodes an E-subgroup PPR protein within the mitochondria. Molecular analyses showed that the editing percentage of 24 RNA editing sites decreased and that of seven RNA editing sites increased in dek55 kernels, the sites of which were distributed across 14 mitochondrial gene transcripts. Moreover, the splicing efficiency of nad1 introns 1 and 4 and nad4 intron 1 significantly decreased in dek55 compared with the wild type (WT). These results indicate that DEK55 plays a crucial role in RNA editing at multiple sites as well as in the splicing of nad1 and nad4 introns. Mutation in the DEK55 gene led to the dysfunction of mitochondrial complex I. Moreover, yeast two-hybrid assays showed that DEK55 interacts with two multiple organellar RNA-editing factors (MORFs), i.e., ZmMORF1 (Zm00001d049043) and ZmMORF8 (Zm00001d048291).Conclusions: Our results demonstrated that a mutation in the DEK55 gene affects the mitochondrial function essential for maize kernel development. Our results also provide novel insight into the molecular functions of E-subgroup PPR proteins involved in plant organellar RNA processing.
The PDC1 gene encoding a pyruvate decarboxylase in S. cerevisiae and Kan r gene were respectively amplified by PCR using oligonucleotides which contained the restriction of NotI, EcoRI, and BglII. The two genes were digested with the same EcoRI and BglII, and linked together for inserting the Kan r gene into the PDC1 gene while the gene disruption cassette was constructed. After transformation of the linear disruption cassette (P1K) into S. cerevisiae Y2, selected transformants were checked by PCR for correct recombination. The haploid mutant Y2-1 △ was obtained, which could increase the yield of pyruvic acid by 176% by shaking flask cultivation as compared with the parental strain Y2.
In this paper, the spatial distributions and seasonal dynamics of soil microbes and microbial biomass were investigated in a typical reed marsh in Zhalong natural wetlands.We wanted to explore the main factors that impacted their spatio-temporal patterns. The results showed that: Bacteria were dominant, followed by actinomyces and fungi were at least in the soil microbes community. The seasonal dynamics of soil microbial biomass carbon and nitrogen were more regularly, and their change patterns were significantly as "W" types. The response of soil microbial biomass in Bottom (10-30cm) to time was slower than the surface, and it fluctuated tinily in every months. The correlation analysis shows that the soil nutrient and soil microbial activity had close relationship. Soil microbial biomass carbon and nitrogen were all significantly positively correlated to quantities of fungus, organic carbon content and Alkali-hytrolyzabel N content(P<0.01), but negative extremely significantly correlated with pH (P<0.01).
Background: Pentatricopeptide repeat (PPR) proteins form a large protein family that participates in RNA processing in organelles and plant growth. Previous reports regard E-subgroup PPR proteins as editing factors for RNA editing. However, additional functions and roles of the E-subgroup PPR proteins remain to be investigated.Results: In this study, we developed and identified a new maize kernel mutant with arrested embryo and endosperm development, i.e., defective kernel 55 (dek55). Genetic and molecular evidence suggested that the defective kernels was a result of a mononucleotide alteration (C to T) at +449 bp in the open reading frame (ORF) of Zm00001d014471 (hereafter referred to as DEK55). DEK55 encodes an E-subgroup PPR protein within mitochondria. Molecular analyses showed that the editing ratio of 24 RNA editing sites was decreased and that of seven RNA editing sites was increased in dek55 mutant kernels, which were distributed in 14 mitochondrial gene transcripts. Meanwhile, the splicing efficiency of the nad1 introns 1 and 4 and nad4 intron 1 was significantly decreased in dek55 compared with that of wild-type (WT). These results indicate that DEK55 plays a crucial role in RNA editing at multiple sites as well as in the splicing of nad1 and nad4 introns. Mutation in the DEK55 gene led to the dysfunction of mitochondrial complex I. Yeast two-hybrid assays showed that the DEK55 interacts with two multiple organellar RNA editing factors (MORFs), i.e., ZmMORF1 (Zm00001d049043) and ZmMORF8 (Zm00001d048291), respectively.Conclusions: Our results demonstrated that a mutation in the DEK55 gene affects the mitochondrial function essential for maize kernel development. Our results also provide novel insight into the molecular functions of the E-subgroup PPR proteins in plant organellar RNA processing.
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