Comparative identification of microRNAs in<i>Apis cerana cerana</i>workers’ midguts responding to<i>Nosema ceranae</i>invasion

Guo, Rui; Chen, Dafu; Du, Yuguang; Chen, Huazhi; Wang, Haipeng; Zheng, Yusheng; Hou, Chunsheng; Diao, Qingyun

doi:10.1101/528166

Cited by 9 publications

(7 citation statements)

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“…1C). The shared miRNA profile is from normal and N. ceranae -infected midguts of A. c. cerana workers [1]. On average, more than 12.54 Mb raw reads in each group were yielded from sRNA-seq, and over 12.02 Mb (95.83%) clean reads were gained after strict filtering and quality control (Table 1).…”

Section: Datamentioning

confidence: 84%

“…Small RNA libraries were constructed according to the general protocol [1]. Briefly, total RNA of each midgut sample in N. ceranae -treated and control groups were extracted using TRIzol Reagent followed by removal of DNA contaminants; only values of 28S/18S ≥ 0.7 and RIN ≥7.0 were considered qualified for the subsequent small RNA library construction.…”

Section: Experimental Design Materials and Methodsmentioning

confidence: 99%

“…Additionally, Pearson correlation coefficients between different biological replicas within each control and N. ceranae -infected group were above 0.9768 and 0.9912, respectively (Fig. 2) [1]. In total, 14 differentially expressed miRNAs (DEmiRNAs) were observed in midgut at 7 days post inoculation (dpi) with N. ceranae (AcT1) compared with corresponding normal midgut (AcCK1), including eight up-regulated and six down-regulated miRNAs (Table 2); while 12 miRNA with differential expressions were detected in midgut at 10 dpi with N. ceranae (AcT2) compared with corresponding normal midgut (AcCK2), including nine up-regulated and three down-regulated ones (Table 3).…”

Section: Datamentioning

confidence: 99%

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MicroRNA dataset of normal and Nosema ceranae-infected midguts of Apis cerana cerana workers

Zhou

Chen

et al. 2019

Data in Brief

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Nosema ceranae is a widespread fungal pathogen of honeybees, which is infective to all castes in the colony, including queens, drones and workers. Nosemosis caused by N. ceranae poses a big challenge for apiculture all over the world. Here, midguts of normal and N. ceranae-infected Apis cerana cerana workers at 7 and 10 days post infection were sequenced utilizing small RNA sequencing (sRNA-seq) technology. Totally, more than 150.54 Mb raw reads were produced in this article, and over 144.26 Mb high-quality clean reads with a mean ratio of 95.83% were obtained after strict filtering and quality control. For more insight please see “Comparative identification of microRNAs in Apis cerana cerana workers' midguts responding to Nosema ceranae invasion” (Chen et al., 2019). Raw data are available in NCBI Sequence Read Archive (SRA) database under the BioProject number PRJNA487111. Our data can be used for investigating differentially expressed microRNAs (miRNAs) and piRNAs and their regulatory roles engaged in A. c. cerana response to N. ceranae infection, and for offering potential candidates for uncovering the molecular mechanisms regulating eastern honeybee-microsporidian interactions.

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Section: Datamentioning

confidence: 84%

Section: Experimental Design Materials and Methodsmentioning

confidence: 99%

Section: Datamentioning

confidence: 99%

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MicroRNA dataset of normal and Nosema ceranae-infected midguts of Apis cerana cerana workers

Zhou

Chen

et al. 2019

Data in Brief

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“…The inoculation and rearing of A. c. cerana workers as well as midgut sample preparation were performed according to the established procedure in our lab [4, 5]. Briefly, (1) To offer newly emerged Nosema-free workers, combs of sealed brood from a healthy colony were kept in an incubator at 34 ± 0.5 °C, 50% RH; the emergent workers were seriously transferred into cages in groups (n=35) and kept in the incubator at 32 ± 0.5 °C, 50% RH.…”

Section: Experimental Design Materials and Methodsmentioning

confidence: 99%

Nanopore-based genome-wide DNA methylation sequencing data of Nosema ceranae-inoculated and un-inoculated eastern honeybee workers’ midguts

Chen

Guo

2021

Preprint

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Apis cerana cerana is an excellent subspecies of Apis cerana, playing a vital role in pollination for wild flowers and crops as well as ecological balance. Nosema ceranae, an emergent fungal parasite infecting various bee species, originates from eastern honeybee. In this article, midguts of N. ceranae-inoculated A. c. cerana workers at 7 days post inoculation (dpi) and 10 dpi (AcT1 and AcT2) and un-inoculated workers’ midguts (AcCK1, AcCK2) were subjected to Nanopore-based genome-wide DNA methylation sequencing. Totally, 1773258, 2151476, 1927874 and 2109961 clean reads were generated from AcCK1, AcCK2, AcT1, and AcT2 groups, with the N50 lengths of 7548, 7936, 7678, and 7291 and the average quality value of 8.97, 8.95, 9.24, and 8.98, respectively. Among these, 93.85%, 94.49%, 88.69%, and 81.27% clean reads could be mapped to the reference genome of A. c. cerana. In the aforementioned four groups, 2149685, 2614513, 1637018 and 2726985 CHG sites were identified; the numbers of CHH sites were 9581990, 11801082, 7178559, and 12342423, whereas those of CpG sites were 14325356, 15703508, 14856284 and 13956849, respectively. Additionally, there were 36114, 118867, 30249, and 82984 6mA methylation sites respectively discovered. These data can be used for identifying differential 5mC methylation and 6mA methylation engaged in response of eastern honeybee workers to N. ceranae infestation, and for investigating the 5mC or 6mA methylation-mediated mechanism underlying host response.Value of the dataThe data provide enrichment for information about 5mC and 6mA methylation in eastern honeybees.Our data contributes to clarification of the epigenetic mechanism underlying eastern honeybee worker’s response to microsporidian infestation.This presented data offer novel insights into interaction between Apis cerana and Nosema ceranae.

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“…MicroRNAs (miRNAs) are a class of small noncoding RNAs of approximately 22 nt in length, which regulate gene expression at the post-transcriptional level by targeting sites in mRNA, and have been shown to regulate a variety of physiological processes throughout insect development [4]. Up to date, thousands of miRNAs have been identi ed from insect species, including Drosophila melanogaster [5], Bombyx mori [6,7], Locusta migratoria [8], Manduca sexta [9][10][11], Plutella xylostella [12,13], Helicoverpa armigera [14,15], Mayetiola destructor [16], Nilaparvata lugens [17], Blattella germanica [18], Aphis gossypii [19], Lissorhoptrus oryzophilus [20], Leptinotarsa decemlineata [21], Grapholita molesta [22], Atrijuglans hetaohei [23], Apis cerana cerana [24], Laodelphax striatellus [25], and Plodia interpunctella [26]. More recent evidence has shown that miRNAs may play an important role in regulation of insect diapause.…”

Section: Introductionmentioning

confidence: 99%

Identification and Comparative Profiling of microRNAs at Different Diapause Stages of Galeruca Daurica Adults

Duan¹,

Li²,

Tan³

et al. 2020

Preprint

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Background: MicroRNAs (miRNAs) are a class of small noncoding RNAs of approximately 22 nt in length, which regulate gene expression at the post-transcriptional level. Although the regulatory roles of miRNAs in various physiological processes throughout insect development have been investigated, it is almost unknown about the roles of miRNAs involved in the regulation of diapause in insects.Results: We constructed 12 small RNA libraries from Galeruca daurica adults at different diapause stages: pre-diapause (PD), diapause (D), post-diapause 1 (TD1), and post-diapause 2 (TD2). Using Illumina sequencing, a total of 95.06 million valid reads was obtained, and 230 miRNAs, including 143 conserved and 87 novel miRNAs, were identified from G. daurica. The expression profiles of these miRNAs were assessed across different diapause stages and miRNAs that were highly expressed at different diapause stages were identified. Comparative analysis of read counts indicated that both conserved and novel miRNAs were differently expressed among the four different diapause stages, and the differential expression was validated via qRT-PCR. The 25, 11, 15, 14, 26, and one miRNAs were differentially expressed in D/PD, D/TD1, D/TD2, TD1/PD, TD2/PD, and TD2/TD1, respectively. The KEGG and GO analysis of the predicted target genes suggested the essential roles of miRNAs in the regulation of summer diapause in G. daurica, especially via the juvenile hormone, ribosome, MAPK signaling, mTOR signaling, Ca2+ signaling, and G-protein coupled receptor signaling pathways.Conclusion: Our research results indicate that miRNAs may be involved in the regulation of summer diapause in G. daurica, and these results also provide an important new small RNA genomics resource for further studies on insect diapause.

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Comparative identification of microRNAs inApis cerana ceranaworkers’ midguts responding toNosema ceranaeinvasion

Cited by 9 publications

References 94 publications

MicroRNA dataset of normal and Nosema ceranae-infected midguts of Apis cerana cerana workers

MicroRNA dataset of normal and Nosema ceranae-infected midguts of Apis cerana cerana workers

Nanopore-based genome-wide DNA methylation sequencing data of Nosema ceranae-inoculated and un-inoculated eastern honeybee workers’ midguts

Identification and Comparative Profiling of microRNAs at Different Diapause Stages of Galeruca Daurica Adults

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Comparative identification of microRNAs inApis cerana ceranaworkers’ midguts responding toNosema ceranaeinvasion

Cited by 9 publications

References 94 publications

MicroRNA dataset of normal and Nosema ceranae-infected midguts of Apis cerana cerana workers

MicroRNA dataset of normal and Nosema ceranae-infected midguts of Apis cerana cerana workers

Nanopore-based genome-wide DNA methylation sequencing data of Nosema ceranae-inoculated and un-inoculated eastern honeybee workers’ midguts

Identification and Comparative Profiling of microRNAs&nbsp;at Different Diapause Stages of Galeruca Daurica Adults

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Identification and Comparative Profiling of microRNAs at Different Diapause Stages of Galeruca Daurica Adults