Your search keyword '"housekeeping genes"' showing total 1,128 results

1. Selection and validation of reference genes for RT-qPCR gene expression studies in Candida viswanathii cultivated under different grown conditions

Author

Daúde, Matheus Martins, Teixeira, Ronan Cristhian, Cardon, Carlos Henrique, de Araujo Santos, Gessi Carvalho, de Almeida, Alex Fernando, Chalfun-Junior, Antonio, and Barreto, Horllys Gomes

Published

2023

2. Reference gene selection for real-time qPCR in European flounder (Platichthys flesus) using organ-specific RNA-seq data.

Author

Pomianowski, Konrad and Burzyński, Artur

Abstract

Background: The European flounder is readily chosen as an experimental subject and model in physiological and ecotoxicological studies mostly because of its adaptability to laboratory conditions. Many studies utilise a quantitative PCR (qPCR) approach to ascertain the expression of target genes under experimental conditions. Such an approach relies heavily on the selection of reference genes with stable expression. Yet certain housekeeping genes are commonly used in this role, often without due consideration of their overall expression patterns. Therefore, new approaches should be developed to identify stable reference genes for a given species and to expand the general pool of genes suitable for the reference in qPCR analysis. Methods and results: Here RNA-seq data of nine flounder organs led to identify four candidate genes of the most stable expression. It was achieved by differential expression analysis and tritoconstrictor script. Specific primers were designed for the complete ORF as well as for qPCR analysis. RT-qPCR efficiencies were tested on ORF amplicon templates. Most of the genes tested showed good amplification in a wide range of template dilutions (107-101), with a correlation coefficient (R2) ranging from 0.991 to 0.998 and a consistent efficiency (E) (Sybr Green I staining and TaqMan molecular probe). Conclusions: The proposed approach based on differential expression analysis and a new bioinformatic tool is an appropriate selection method of candidates for reference genes in qPCR. The proposed approach, combining differential expression analysis with a new bioinformatics tool, provides an effective method for selecting reference gene candidates for qPCR. As a result, we can propose four genes (polr2f, yif1a, sf3b6, uba52), each with a set of validated primers, as suitable for consideration as reference genes in qPCR analysis in European flounder, an emerging model species. [ABSTRACT FROM AUTHOR]

Published

2025

3. Wolbachia of phylogenetic supergroup K identified in oribatid mite Nothrus anauniensis (Acari: Oribatida: Nothridae).

Author

Kang, Shuo-Fang, Chen, Yu, and Chen, Jun

Subjects

CYTOPLASMIC inheritance, GENITALIA, WOLBACHIA, ACARIFORMES, MITES, ORIBATIDAE

Abstract

Heritable endosymbionts widely occur in arthropod and nematode hosts. Among these endosymbionts, Wolbachia has been extensively detected in many arthropods, such as insects and crustaceans. Maternal inheritance is the most basic and dominant mode of transmission of Wolbachia, and it might regulate the reproductive system of the host in four ways: feminization, parthenogenesis, male killing, and cytoplasmic incompatibility. There is a relatively high percentage (10%) of thelytokous species in Oribatida, a suborder under the subclass Acari of arthropods, but the study of the endosymbionts in oribatid mites is almost negligible. In this paper, we detected endosymbiotic bacteria in two parthenogenetic oribatid species, Nothrus anauniensis Canestrini and Fanzago, 1877, which has never been tested for endosymbionts, and Oppiella nova, in which Wolbachia and Cardinium have been reported before. The results showed that Wolbachia was first found in N. anauniensis with an infection rate of 100% across three populations. Phylogenetic analysis showed that Wolbachia in N. anauniensis belonged to the supergroup K, marking the second supergroup of Wolbachia found in oribatid mites. Unlike previous studies, our study did not detect Wolbachia in O. nova, leading to the exclusion of Wolbachia's role in mediating thelytoky in this species. [ABSTRACT FROM AUTHOR]

Published

2024

4. Phylogenetic diversity of Rhizobium species recovered from nodules of common beans (Phaseolus vulgaris L.) in fields in Uganda: R. phaseoli, R. etli, and R. hidalgonense.

Author

Aserse, Aregu Amsalu, Nimusiima, Jean, Tumuhairwe, John Baptist, Yli-Halla, Markku, and Lindström, Kristina

Subjects

*HORIZONTAL gene transfer, *NITROGEN fixation, *SPECIES distribution, *SPECIES diversity, *ENVIRONMENTAL sampling

Abstract

A total of 75 bacterial isolates were obtained from nodules of beans cultivated across 10 sites in six agro-ecological zones in Uganda. Using recA gene sequence analysis, 66 isolates were identified as members of the genus Rhizobium , while 9 were related to Agrobacterium species. In the recA gene tree, most Rhizobium strains were classified into five recognized species. Phylogenetic analysis based on six concatenated sequences (r ecA–rpoB–dnaK–glnII–gyrB–atpD) placed 32 representative strains into five distinct Rhizobium species, consistent with the species groups observed in the recA gene tree: R. phaseoli, R. etli, R. hidalgonense, R. ecuadorense , and R. sophoriradicis , with the first three being the predominant. The rhizobial strains grouped into three nodC subclades within the symbiovar phaseoli clade, encompassing strains from distinct phylogenetic groups. This pattern reflects the conservation of symbiotic genes, likely acquired through horizontal gene transfer among diverse rhizobial species. The 32 representative strains formed symbiotic relationships with host beans, while the Agrobacterium strains did not form nodules and lacked symbiotic genes. Multivariate analysis revealed that species distribution was influenced by the environmental factors of the sampling sites, emphasizing the need to consider these factors in future effectiveness studies to identify effective nitrogen-fixing strains for specific locations. [ABSTRACT FROM AUTHOR]

Published

2024

5. Screening and validating the optimal panel of housekeeping genes for 4T1 breast carcinoma and metastasis studies in mice.

Author

Souza, Jorge Lucas Nascimento, Antunes-Porto, Ana Rafaela, da Silva Oliveira, Izabela, Amorim, Chiara Cássia Oliveira, Pires, Luiz Octávio, de Brito Duval, Isabela, Amaral, Luisa Vitor Braga do, Souza, Fernanda Rezende, Oliveira, Evelyn Ane, Cassali, Geovanni Dantas, Cardoso, Valbert Nascimento, Fernandes, Simone Odília Antunes, Fujiwara, Ricardo Toshio, Russo, Remo Castro, and Bueno, Lilian Lacerda

Subjects

*ANIMAL tracks, *TRIPLE-negative breast cancer, *MOLECULAR biology, *GENE expression, *BREAST cancer, *BREAST

Abstract

The 4T1 model is extensively employed in murine studies to elucidate the mechanisms underlying the carcinogenesis of triple-negative breast cancer. Molecular biology serves as a cornerstone in these investigations. However, accurate gene expression analyses necessitate data normalization employing housekeeping genes (HKGs) to avert spurious results. Here, we initially delve into the characteristics of the tumor evolution induced by 4T1 in mice, underscoring the imperative for additional tools for tumor monitoring and assessment methods for tracking the animals, thereby facilitating prospective studies employing this methodology. Subsequently, leveraging various software platforms, we assessed ten distinct HKGs (GAPDH, 18 S, ACTB, HPRT1, B2M, GUSB, PGK1, CCSER2, SYMPK, ANKRD17) not hitherto evaluated in the 4T1 breast cancer model, across tumors and diverse tissues afflicted by metastasis. Our principal findings underscore GAPDH as the optimal HKG for gene expression analyses in tumors, while HPRT1 emerged as the most stable in the liver and CCSER2 in the lung. These genes demonstrated consistent expression and minimal variation among experimental groups. Furthermore, employing these HKGs for normalization, we assessed TNF-α and VEGF expression in tissues and discerned significant disparities among groups. We posit that this constitutes the inaugural delineation of an ideal HKG for experiments utilizing the 4T1 model, particularly in vivo settings. [ABSTRACT FROM AUTHOR]

Published

2024

6. Development of RT-qPCR assay for assessing the expression of ACTB and SDHA housekeeping genes in the cell cultures of mammalian hosts of zoonotic infections

Author

N. A. Liapunova, M. A. Khasnatinov, G. A. Danchinova, and I. S. Solovarov

Subjects

apodemus peninsulae, sus scrofa, cell lines, expression, mrna, sdha, actb, housekeeping genes, quantitative rt-pcr, Science

Abstract

Background. The molecular mechanisms behind the maintenance of zoonotic pathogens in nature can be better understood by examining the gene expression in host cells in response to the infection. Reverse transcription and quantitative polymerase chain reaction (RT-qPCR) is a powerful method to study gene expression, especially with the use of endogenous reference genes (RG) to normalize the data. Therefore, it is critical to develop the reliable qRT-PCR assay and validate that selected RGs are stably expressed in the studied organism or cell culture.The aim. In this work, we aimed to develop the real-time qRT-PCR method for detecting mRNA of two candidate RGs, succinate dehydrogenase subunit A (SDHA) and beta-actin (ACTB), in the cell lines of mammalian hosts of zoonotic infections.Materials and methods. The SPEV (porcine embryonic kidney cell line) and ApnK (Korean field mouse kidney cell line) cells were grown in 24-well culture plates. Total RNA/DNA was isolated from trypsin-detached cell monolayers. Genomic DNA in the samples was removed with RNase-free DNase I, and one-step RT-qPCR was performed using primers for SDHA and ACTB gene fragments and the corresponding TaqMan hydrolysis probes. The experiment was performed in 4 independent replicates.Results. In the Korean field mouse cells, the linearity, efficiency, repeatability, and reproducibility of the RT-qPCR for ACTB gene mRNA corresponded to the modern requirements. However, RT-qPCR for SDHA exhibited good linearity and efficiency of the reaction, but CV values for repeatability and reproducibility slightly exceeded the recommended standards. In porcine cells, both assays had acceptable parameters. Thus, to use the SDHA as RG for ApnK cells, a detailed study of the stability of its expression in this particular model is required.Conclusions. New qRT-PCR assay was developed to assess the expression of housekeeping genes ACTB and SDHA in the cells of the Korean field mouse and domestic pig. Further research is necessary to validate these genes as references for quantitative assessment of gene expression in the cells of mammalian hosts of zoonotic infections.

Published

2024

7. Screening and validating the optimal panel of housekeeping genes for 4T1 breast carcinoma and metastasis studies in mice

Author

Jorge Lucas Nascimento Souza, Ana Rafaela Antunes-Porto, Izabela da Silva Oliveira, Chiara Cássia Oliveira Amorim, Luiz Octávio Pires, Isabela de Brito Duval, Luisa Vitor Braga do Amaral, Fernanda Rezende Souza, Evelyn Ane Oliveira, Geovanni Dantas Cassali, Valbert Nascimento Cardoso, Simone Odília Antunes Fernandes, Ricardo Toshio Fujiwara, Remo Castro Russo, and Lilian Lacerda Bueno

Subjects

Housekeeping genes, Gene expression, Experimental metastasis, RT-qPCR, Radioisotopes, Medicine, Science

Abstract

Abstract The 4T1 model is extensively employed in murine studies to elucidate the mechanisms underlying the carcinogenesis of triple-negative breast cancer. Molecular biology serves as a cornerstone in these investigations. However, accurate gene expression analyses necessitate data normalization employing housekeeping genes (HKGs) to avert spurious results. Here, we initially delve into the characteristics of the tumor evolution induced by 4T1 in mice, underscoring the imperative for additional tools for tumor monitoring and assessment methods for tracking the animals, thereby facilitating prospective studies employing this methodology. Subsequently, leveraging various software platforms, we assessed ten distinct HKGs (GAPDH, 18 S, ACTB, HPRT1, B2M, GUSB, PGK1, CCSER2, SYMPK, ANKRD17) not hitherto evaluated in the 4T1 breast cancer model, across tumors and diverse tissues afflicted by metastasis. Our principal findings underscore GAPDH as the optimal HKG for gene expression analyses in tumors, while HPRT1 emerged as the most stable in the liver and CCSER2 in the lung. These genes demonstrated consistent expression and minimal variation among experimental groups. Furthermore, employing these HKGs for normalization, we assessed TNF-α and VEGF expression in tissues and discerned significant disparities among groups. We posit that this constitutes the inaugural delineation of an ideal HKG for experiments utilizing the 4T1 model, particularly in vivo settings.

Published

2024

8. Expression patterns of housekeeping genes and tissue-specific genes in black goats across multiple tissues

Author

Chaobin Qin, Dong Wang, Hongbing Han, Yanhong Cao, Xiaobo Wang, Zeyi Xuan, Mingsong Wei, Zhipeng Li, and Qingyou Liu

Subjects

Gene expression, Tissue-specific genes, Housekeeping genes, Hub genes, Different feeding methods for black goats, Medicine, Science

Abstract

Abstract Black goats are a significant meat breed in southern China. To investigate the expression patterns and biological functions of genes in various tissues of black goats, we analyzed housekeeping genes (HKGs), tissue-specific genes (TSGs), and hub genes (HUBGs) across 23 tissues. Additionally, we analyzed HKGs in 13 tissues under different feeding conditions. We identified 2968 HKGs, including six important ones. Interestingly, HKGs in grazing black goats demonstrated higher and more stable expression levels. We discovered a total of 9912 TSGs, including 134 newly identified ones. The number of TSGs for mRNA and lncRNA were nearly equal, with 127 mRNA TSGs expressed solely in one tissue. Additionally, the predicted functions of tissue-specific long non-coding RNAs (lncRNAs) targeting mRNAs corresponded with the physiological functions of the tissues.Weighted gene co-expression network analysis (WGCNA) constructed 30 modules, where the dark grey module consists almost entirely of HKGs, and TSGs are located in modules most correlated with their respective tissues. Additionally, we identified 289 HUBGs, which are involved in regulating the physiological functions of their respective tissues. Overall, these identified HKGs, TSGs, and HUBGs provide a foundation for studying the molecular mechanisms affecting the genetic and biological processes of complex traits in black goats.

Published

2024

9. Assessment of housekeeping genes stability for gene transcription regulation analysis of Spodoptera littoralis (Lepidoptera: Noctuidae) under Spodoptera littoralis nucleopolyhedrovirus viral infection.

Author

Elmenofy, Wael, Abdelsattar, Mohamed, Kesba, Hosny H., and El-Maksoud, Reem M. Abd

Abstract

Background: Normalization with respect to stable housekeeping genes is important to facilitate gene transcription regulation research and acquire more accurate quantitative polymerase chain reaction (qPCR) data. In the current study, five candidates housekeeping genes of the cotton leafworm, Spodoptera littoralis encoding for Actin (Actin), elongation factor 1-alpha (EF1α), ribosomal protein S3 (RPS3), ribosomal protein 49 (RP49), and Ubiquitin (Ubi), were evaluated as normalization housekeeping genes under Spodoptera littoralis nucleopolyhedrovirus (SpliNPV) viral infection. Methods and Results: The qPCR results confirmed the expression of all five housekeeping genes in S. littoralis viral infected larvae. The expression profiles of the housekeeping genes showed that the EF1α, Actin, and RP49 had the minimum average Ct values of 18.41 ± 0.66, 18.84 ± 0.90 and 19.01 ± 0.87 in all infected samples, respectively. While RPS3 and Ubi showed the maximum average Ct of 21.61 ± 0.51 and 21.11 ± 0.82, respectively. According to the results of ΔCt and geNorm analysis, EF1α was ranked as the most stable housekeeping gene during infection time-course. While by using BestKeeper, geNorm and NormFinder, the Ubi, RP49, and RPS3 showed the most genes transcription stability. The obtained results were also validated using the Cytochrome c oxidase (COX) gene transcripts in response to SpliNPV infection. Conclusions: The results revealed that EF1α and Ubi were the most stable housekeeping genes to be used for normalizing S. littoralis gene transcription regulation under SpliNPV infection. These findings, provide a significant addition for gene transcription regulation studies of S. littoralis upon infection using SpliNPV as a bio-agent. [ABSTRACT FROM AUTHOR]

Published

2024

10. A systematic review on the selection of reference genes for gene expression studies in rodents: are the classics the best choice?

Author

Bunde, Tiffany T., Pedra, Ana C. K., de Oliveira, Natasha R., Dellagostin, Odir A., and Bohn, Thaís L. O.

Abstract

Rodents are commonly used as animal models in studies investigating various experimental conditions, often requiring gene expression analysis. Quantitative real-time reverse transcription PCR (RT-qPCR) is the most widely used tool to quantify target gene expression levels under different experimental conditions in various biological samples. Relative normalization with reference genes is a crucial step in RT-qPCR to obtain reliable quantification results. In this work, the main reference genes used in gene expression studies among the three rodents commonly employed in scientific research—hamster, rat, and mouse—are analyzed and described. An individual literature search for each rodent was conducted using specific search terms in three databases: PubMed, Scopus, and Web of Science. A total of 157 articles were selected (rats = 73, mice = 79, and hamsters = 5), identifying various reference genes. The most commonly used reference genes were analyzed according to each rodent, sample type, and experimental condition evaluated, revealing a great variability in the stability of each gene across different samples and conditions. Classic genes, which are expected to be stably expressed in both samples and conditions analyzed, demonstrated greater variability, corroborating existing concerns about the use of these genes. Therefore, this review provides important insights for researchers seeking to identify suitable reference genes for their validation studies in rodents. [ABSTRACT FROM AUTHOR]

Published

2024

11. Selecting reference genes for RT-qPCR studies involving the presence of B chromosomes in Psalidodon (Characiformes, Characidae).

Author

Vidal, Mateus Rossetto, Lasmar, Lucas F., Nadai, Pamela C. F., Oliveira, Claudio, Silva, Duilio M. Z. A., and Foresti, Fausto

Abstract

Background: B chromosomes are extra non-essential elements present in several eukaryotes. Unlike A chromosomes which are essential and present in all individuals of a species, B chromosomes are not necessary for normal functioning of an organism. Formerly regarded as genetically inactive, B chromosomes have been discovered to not only express their own genes, but also to exert influence on gene expression in A chromosomes. Recent studies have shown that, in some Psalidodon (Characiformes, Characidae) species, B chromosomes might be associated with phenotypic effects, such as changes in the reproductive cycle and gene expression. Methods and results: In this study, we aimed to establish stable reference genes for RT-qPCR experiments conducted on gonads of three fish species within Psalidodon genus, both in the presence and absence of B chromosomes. The stability of five selected reference genes was assessed using NormFinder, geNorm, BestKeeper, and RefFinder algorithms. We determined ppiaa and pgk1 as the most stable genes in P. fasciatus, whereas ppiaa and hmbsa showed the highest stability in P. bockmanni. For P. paranae, tbp and hprt1 were the most stable genes in females, and ppiaa and hprt1 were the most stable in males. Conclusions: We determined the most stable reference genes in gonads of three Psalidodon species considering the presence of B chromosomes. This is the first report of reference gene stability in the genus and provides valuable tools to better understand the effects of B chromosomes at gene expression level. [ABSTRACT FROM AUTHOR]

Published

2024

12. CHD6 eviction of promoter nucleosomes maintains housekeeping transcriptional program in prostate cancer

Author

Lina Bu, Shaodong Huang, Ziyan Rao, Chenyang Wu, Bryan-Yu Sun, Yanhua Liu, Lin He, and Dongyu Zhao

Subjects

MT: Bioinformatics, CHD6, housekeeping genes, histone modifications, epigenetics, chromatin remodeling, Therapeutics. Pharmacology, RM1-950

Abstract

CHD6, a member of the chromodomain helicase DNA-binding protein family, has been implicated in various diseases and tumors. However, its precise binding model of CHD6 on regulatory functional genes remains poorly understood. In this study, we discovered sharp peaks of CHD6, as the first member of CHD family for housekeeping process, binding only to the promoter region of genes in the C4-2 cell line. These genes, with conserved sharp CHD6 peaks across tumor cells, likely represent housekeeping genes ADNP and GOLGA5. Genes with sharp CHD6 peaks exhibit stable and low expression levels, sharing epigenetic features similar to housekeeping genes. Furthermore, this regulatory model also exists in both HEK293 cells and cardiomyocytes. Overall, the results of this study demonstrate that CHD6 binds to the promoter regions of housekeeping genes, regulating their histone modifications, chromatin structure, and gene expression.

Published

2024

13. Contact lenses as novel tear fluid sampling vehicles for total RNA isolation, precipitation, and amplification

Author

Nikolay Boychev, Seokjoo Lee, Vincent Yeung, Amy E. Ross, Liangju Kuang, Lin Chen, Reza Dana, and Joseph B. Ciolino

Subjects

Tear fluid, RNA, Contact lenses, Housekeeping genes, Biomarkers, Ocular diseases, Medicine, Science

Abstract

Abstract The tear fluid is a readily accessible, potential source for biomarkers of disease and could be used to monitor the ocular response to contact lens (CL) wear or ophthalmic pathologies treated by therapeutic CLs. However, the tear fluid remains largely unexplored as a biomarker source for RNA-based molecular analyses. Using a rabbit model, this study sought to determine whether RNA could be collected from commercial CLs and whether the duration of CL wear would impact RNA recovery. The results were referenced to standardized strips of filtered paper (e.g., Shirmer Strips) placed in the inferior fornix. By performing total RNA isolation, precipitation, and amplification with commercial kits and RT-PCR methods, CLs were found to have no significant differences in RNA concentration and purity compared to Schirmer Strips. The study also identified genes that could be used to normalize RNA levels between tear samples. Of the potential control genes or housekeeping genes, GAPDH was the most stable. This study, which to our knowledge has never been done before, provides a methodology for the detection of RNA and gene expression changes from tear fluid that could be used to monitor or study eye diseases.

Published

2024

14. Housekeeping protein-coding genes interrogated with tissue and individual variations

Author

Kuo-Feng Tung, Chao-Yu Pan, and Wen-chang Lin

Subjects

Protein-coding gene, Housekeeping genes, GTEx project, Next-generation sequencing, Gini index, Medicine, Science

Abstract

Abstract Housekeeping protein-coding genes are stably expressed genes in cells and tissues that are thought to be engaged in fundamental cellular biological functions. They are often utilized as normalization references in molecular biology research and are especially important in integrated bioinformatic investigations. Prior studies have examined human housekeeping protein-coding genes by analyzing various gene expression datasets. The inclusion of different tissue types significantly impacted the discovery of housekeeping genes. In this report, we investigated particularly individual human subject expression differences in protein-coding genes across different tissue types. We used GTEx V8 gene expression datasets obtained from more than 16,000 human normal tissue samples. Furthermore, the Gini index is utilized to investigate the expression variations of protein-coding genes between tissue and individual donor subjects. Housekeeping protein-coding genes found using Gini index profiles may vary depending on the tissue subtypes investigated, particularly given the diverse sample size collections across the GTEx tissue subtypes. We subsequently selected major tissues and identified subsets of housekeeping genes with stable expression levels among human donors within those tissues. In this work, we provide alternative sets of housekeeping protein-coding genes that show more consistent expression patterns in human subjects across major solid organs. Weblink: https://hpsv.ibms.sinica.edu.tw .

Published

2024

15. A Comparison of GAPDH and ACTB As Internal Control for Gene Expression Studies in Different Cancer Cell Lines.

Author

KOSE, Tugba

Subjects

*GLYCERALDEHYDEPHOSPHATE dehydrogenase, *TISSUE inhibitors of metalloproteinases, *GENE expression, *CELL lines, *INTERNAL auditing

Abstract

Housekeeping genes are used as internal controls to normalize the expression of target genes in gene expression studies. Glyceraldehyde 3-phosphate dehydrogenase (GAPDH) and Actin beta (ACTB) are frequently preferred as housekeeping genes in gene expression studies. Due to the general alterations in the gene expression pattern in cancer cases, the selection of the appropriate housekeeping genes for these studies are challenging. In this study, we aimed to analyze the expression of the well-known housekeeping genes GAPDH and ACTB in 6 different cancer cell lines. Furthermore, the relative gene expression of the selected target gene (Tissue inhibitor of metalloproteinases 2-TIMP2) was normalized separately using GAPDH and ACTB and the obtained results were compared with each other. Finally, the stability of GAPDH and ACTB was analyzed using the in-silico tool, Bestkeeper. As a result of the study, it is found that the expression of GAPDH and ACTB were significantly different in the Jurkat (p< 0.01), MOLT4 (p< 0.05), REH (p< 0.001) and HT29 (p< 0.001) cell lines. Based on this finding, significantly different relative target gene expression values were obtained in different cell lines depending on whether the selected housekeeping gene was GAPDH or ACTB. In addition, GAPDH was found to show less variation among the samples used in all cell lines and more stability based on Bestkeeper analysis. These results support that the appropriate housekeeping gene selection, especially in cancer cell lines, may be an effective factor in obtaining accurate results for the studies in the field provide guidance to researchers. [ABSTRACT FROM AUTHOR]

Published

2024

16. Reliable detection of RNA in hippocampus sections of mice by FISH up to a post-mortem delay of 24 h.

Author

Seiffer, Sophie, Brendler, Jana, Schulz, Angela, and Ricken, Albert

Subjects

*RNA, *HIPPOCAMPUS (Brain), *G protein coupled receptors, *PROTEIN receptors

Abstract

Proteins can be successfully localized in post-mortem (PM) brain tissue sections if the time until PM tissue sampling is not too long. In this study, we show that this also applies to the localization of RNA and in particular to the RNA of microglia-specific receptor proteins using the probes and the RNAscope™ Multiplex Fluorescent Detection Kit v2 from Advanced Cell Diagnostics. Brains were removed from killed mice after different PM delays and processed into paraffin sections. In sections of brains from animals whose cadavers had been kept at room temperature (21 °C) before tissue removal, ubiquitously expressed RNAs of genes with low to high expression levels (Polr2a, PPIB, and UBC) were reliably detected in the brain sections even if tissue removal was delayed by up to 48 h. In addition, microglia-specific G protein-coupled receptor RNA (Gpr34, P2ry12) could be reliably assigned to microglia by simultaneous labeling of the microglia with microglia-specific antibodies (Iba1 or P2ry12). Only after a delay of 48 h until tissue removal were the receptor RNA signals significantly lower. The reduction in receptor RNA signals could be delayed if the animal cadavers were stored at 4 °C until the brains were removed. Tissue sections of PM brain samples allow the spatial and cellular localization of specific RNA, at least if the sampling takes place within the first 24 h of PM. [ABSTRACT FROM AUTHOR]

Published

2024

17. Screening and Stability Analysis of Housekeeping Genes for Transcriptomic Studies in Danio rerio (Zebrafish) at Early Developmental Stages.

Author

Partevian, S. A., Safina, D. R., Rybolovlev, I. N., Rudenok, M. M., Kostrov, S. V., Shadrina, M. I., Slominsky, P. A., and Alieva, A. Kh.

Abstract

The zebrafish (Danio rerio) is one of the promising objects for modeling pathological conditions. A large number of such works are carried out at the transcriptomic level. Transcriptomic studies require the use of stable housekeeping genes (HKGs), and so we selected candidate HKGs and analyzed their stability in D. rerio under normal conditions. The work was carried out using D. rerio of the AB line whose embryos were sampled at three time points: the hatching stage (2 days postfertilization, dpf), and early larval stages (5 and 9 dpf). Analysis of HKG expression levels was performed using real-time polymerase chain reaction. Further analysis of the obtained Ct results was carried out in the RefFinder program. Different HKGs are suitable for assessing changes in gene expression at different stages of D. rerio development. When assessing changes in gene expression at the hatching stage (2 dpf), the optimal pair of HKGs is aars1 and polr2f; for the early larval stage (5 dpf), it is aars1 and psmd6; and for 9 dpf, it is bcat2 and actb1. During transcriptomic studies conducted at several developmental stages simultaneously, it is necessary to use a single selected pair of HKGs for all the studied stages of zebrafish development: aars1 and lsm12b. According to the data obtained, aars1 and lsm12b are the most stable HKGs for all the early developmental stages of D. rerio studied. At the same time, we first showed that aars1 is the most stable HKG for the early stages of the development. The second most stable HKG is lsm12b. Our data on the stability of the lsm12b gene are consistent with previously published data. [ABSTRACT FROM AUTHOR]

Published

2024

18. Housekeeping protein-coding genes interrogated with tissue and individual variations.

Author

Tung, Kuo-Feng, Pan, Chao-Yu, and Lin, Wen-chang

Subjects

*HOUSEKEEPING, *GENE expression, *GENES, *TISSUES, *CELL physiology

Abstract

Housekeeping protein-coding genes are stably expressed genes in cells and tissues that are thought to be engaged in fundamental cellular biological functions. They are often utilized as normalization references in molecular biology research and are especially important in integrated bioinformatic investigations. Prior studies have examined human housekeeping protein-coding genes by analyzing various gene expression datasets. The inclusion of different tissue types significantly impacted the discovery of housekeeping genes. In this report, we investigated particularly individual human subject expression differences in protein-coding genes across different tissue types. We used GTEx V8 gene expression datasets obtained from more than 16,000 human normal tissue samples. Furthermore, the Gini index is utilized to investigate the expression variations of protein-coding genes between tissue and individual donor subjects. Housekeeping protein-coding genes found using Gini index profiles may vary depending on the tissue subtypes investigated, particularly given the diverse sample size collections across the GTEx tissue subtypes. We subsequently selected major tissues and identified subsets of housekeeping genes with stable expression levels among human donors within those tissues. In this work, we provide alternative sets of housekeeping protein-coding genes that show more consistent expression patterns in human subjects across major solid organs. Weblink: https://hpsv.ibms.sinica.edu.tw. [ABSTRACT FROM AUTHOR]

Published

2024

19. Stability Analysis of Reference Genes for qPCR Studies in Chenopodium quinoa Ecotypes on Salt-Affected Soils.

Author

Triki, Tebra, Boussora, Faiza, Drine, Sawsen, Ben Ali, Sihem, Gasmi, Amel, Bennani, Leila, Marzougui, Nidhal, Ferchichi, Ali, and Guasmi, Ferdaous

Subjects

*QUINOA, *GENE expression, *UBIQUITIN-conjugating enzymes, *FOOD crops, *GENES, *SOIL salinity

Abstract

Soil salinity is one of the most brutal environmental factors that affect crop growth and productivity. Chenopodium quinoa is known as one of the essential food crops in the future due to its agronomic and nutritive value and its strong adaptability to stress environments and soil conditions. However, the molecular aspects of salt tolerance of quinoa remain not well known. Therefore, the expression study of candidate genes related to salt tolerance has become one of the most important features for the identification of their functions. However, one of the most crucial points in Quantitative PCR (qPCR) data analysis is the selection of appropriate reference gene that should be stable and unaffected in a given condition. In this study, six candidate reference genes were analysed in order to select the most stable one under salt stress conditions. The expression stability was assessed using three different algorithms: geNorm, NormFinder and BestKeeper. The most stable and appropriate reference genes screened in this study whose expression was confirmed to be constant in different salt treated and untreated quinoa plant were Monensin sensitivity1 (MON1) and Glyceraldehyde-3-phosphate dehydrogenase (GAPDH) and Factor elongation 1-alpha (EF-1α), while Ubiquitin-conjugating enzyme (UBC) and Ubiquitin-protein ligase 7 (UPL7) had the worst stability. However, the data obtained by BestKeeper demonstrated slight differences compared to those from geNorm and NormFinder. Overall, we designated MON1 and GAPDH as the best candidates and the most stable housekeeping gene under salt stress conditions and their geometric means would provide accurate normalization factor for expression data in Chenopodium quinoa. [ABSTRACT FROM AUTHOR]

Published

2024

20. Multilocus Gene Characterization of Phytoplasmas

Author

Reddy, Madem Gurivi, Rao, Govind Pratap, Singh, Vaibhav Kumar, editor, Akhtar, Jameel, editor, and Singh, Krishna Pratap, editor

Published

2024

21. Expression patterns of housekeeping genes and tissue-specific genes in black goats across multiple tissues

Author

Qin, Chaobin, Wang, Dong, Han, Hongbing, Cao, Yanhong, Wang, Xiaobo, Xuan, Zeyi, Wei, Mingsong, Li, Zhipeng, and Liu, Qingyou

Published

2024

22. Contact lenses as novel tear fluid sampling vehicles for total RNA isolation, precipitation, and amplification

Author

Boychev, Nikolay, Lee, Seokjoo, Yeung, Vincent, Ross, Amy E., Kuang, Liangju, Chen, Lin, Dana, Reza, and Ciolino, Joseph B.

Published

2024

23. Developmental and Housekeeping Genes: Two Types of Genetic Organization in the Drosophila Genome.

Author

Zhimulev, Igor, Vatolina, Tatyana, Levitsky, Victor, and Tsukanov, Anton

Subjects

*CHROMOSOME structure, *DROSOPHILA, *LIFE cycles (Biology), *GENES, *DROSOPHILA melanogaster

Abstract

We developed a procedure for locating genes on Drosophila melanogaster polytene chromosomes and described three types of chromosome structures (gray bands, black bands, and interbands), which differed markedly in morphological and genetic properties. This was reached through the use of our original methods of molecular and genetic analysis, electron microscopy, and bioinformatics data processing. Analysis of the genome-wide distribution of these properties led us to a bioinformatics model of the Drosophila genome organization, in which the genome was divided into two groups of genes. One was constituted by 65, in which the genome was divided into two groups, 62 genes that are expressed in most cell types during life cycle and perform basic cellular functions (the so-called "housekeeping genes"). The other one was made up of 3162 genes that are expressed only at particular stages of development ("developmental genes"). These two groups of genes are so different that we may state that the genome has two types of genetic organization. Different are the timings of their expression, chromatin packaging levels, the composition of activating and deactivating proteins, the sizes of these genes, the lengths of their introns, the organization of the promoter regions of the genes, the locations of origin recognition complexes (ORCs), and DNA replication timings. [ABSTRACT FROM AUTHOR]

Published

2024

24. The Dynamic Interplay Between Ribosomal DNA and Transposable Elements: A Perspective From Genomics and Cytogenetics.

Author

Garcia, Sònia, Kovarik, Ales, Maiwald, Sophie, Mann, Ludwig, Schmidt, Nicola, Pascual-Díaz, Joan Pere, Vitales, Daniel, Weber, Beatrice, and Heitkam, Tony

Subjects

CYTOGENETICS, TRANSPOSONS, DNA insertion elements, GENOMICS, DNA methylation, RIBOSOMAL DNA, HISTONE methylation, EPIGENOMICS

Abstract

Although both are salient features of genomes, at first glance ribosomal DNAs and transposable elements are genetic elements with not much in common: whereas ribosomal DNAs are mainly viewed as housekeeping genes that uphold all prime genome functions, transposable elements are generally portrayed as selfish and disruptive. These opposing characteristics are also mirrored in other attributes: organization in tandem (ribosomal DNAs) versus organization in a dispersed manner (transposable elements); evolution in a concerted manner (ribosomal DNAs) versus evolution by diversification (transposable elements); and activity that prolongs genomic stability (ribosomal DNAs) versus activity that shortens it (transposable elements). Re-visiting relevant instances in which ribosomal DNA–transposable element interactions have been reported, we note that both repeat types share at least four structural and functional hallmarks: (1) they are repetitive DNAs that shape genomes in evolutionary timescales, (2) they exchange structural motifs and can enter co-evolution processes, (3) they are tightly controlled genomic stress sensors playing key roles in senescence/aging, and (4) they share common epigenetic marks such as DNA methylation and histone modification. Here, we give an overview of the structural, functional, and evolutionary characteristics of both ribosomal DNAs and transposable elements, discuss their roles and interactions, and highlight trends and future directions as we move forward in understanding ribosomal DNA–transposable element associations. [ABSTRACT FROM AUTHOR]

Published

2024

25. Stable Housekeeping Genes in Bone Marrow, Adipose Tissue, and Amniotic Membrane-Derived Mesenchymal Stromal Cells for Orthopedic Regenerative Medicine Approaches.

Author

Ragni, Enrico, Piccolo, Simona, Papait, Andrea, De Luca, Paola, Taiana, Michela, Grieco, Giulio, Silini, Antonietta Rosa, Parolini, Ornella, and de Girolamo, Laura

Subjects

*STROMAL cells, *BONE marrow, *AMNION, *HOUSEKEEPING, *CELL populations, *REGENERATIVE medicine

Abstract

The therapeutic effect of mesenchymal stromal cells (MSCs) has been described for a variety of disorders, including those affecting musculoskeletal tissues. In this context, the literature reports several data about the regenerative effectiveness of MSCs derived from bone marrow, adipose tissue, and an amniotic membrane (BMSCs, ASCs, and hAMSCs, respectively), either when expanded or when acting as clinical-grade biologic pillars of products used at the point of care. To date, there is no evidence about the superiority of one source over the others from a clinical perspective. Therefore, a reliable characterization of the tissue-specific MSC types is mandatory to identify the most effective treatment, especially when tailored to the target disease. Because molecular characterization is a crucial parameter for cell definition, the need for reliable normalizers as housekeeping genes (HKGs) is essential. In this report, the stability levels of five commonly used HKGs (ACTB, EF1A, GAPDH, RPLP0, and TBP) were sifted into BMSCs, ASCs, and hAMSCs. Adult and fetal/neonatal MSCs showed opposite HKG stability rankings. Moreover, by analyzing MSC types side-by-side, comparison-specific HKGs emerged. The effect of less performant HKG normalization was also demonstrated in genes coding for factors potentially involved in and predicting MSC therapeutic activity for osteoarthritis as a model musculoskeletal disorder, where the choice of the most appropriate normalizer had a higher impact on the donors rather than cell populations when compared side-by-side. In conclusion, this work confirms HKG source-specificity for MSCs and suggests the need for cell-type specific normalizers for cell source or condition-tailored gene expression studies. [ABSTRACT FROM AUTHOR]

Published

2024

26. Inflammation and Starvation Affect Housekeeping Gene Stability in Adipose Mesenchymal Stromal Cells

Author

Enrico Ragni, Simona Piccolo, Michela Taiana, Caterina Visconte, Giulio Grieco, and Laura de Girolamo

Subjects

mesenchymal stromal cells, housekeeping genes, inflammation, starvation, regenerative medicine, osteoarthritis, Biology (General), QH301-705.5

Abstract

Due to the scientific success of in vitro and in vivo model studies, the interest in using mesenchymal stromal cells (MSCs) for the treatment of orthopaedic conditions is growing. In the context of osteoarthritis (OA), MSCs, and, in particular, those derived from adipose tissues (ASCs), have found broader access to clinical use as active components of minimally manipulated orthobiologics, as well as clinically expanded cell preparations, or to collect their released factors (secretome) for cell-free approaches. In this regard, while both inflammatory priming and starvation are common strategies used to empower cell potency or collect the secretome, respectively, little is known about the possible influence of these approaches on the stability of housekeeping genes (HKGs) for molecular studies able to fingerprint cell phenotype or potency. In this report, the reliability of five commonly used HKGs (ACTB, B2M, GAPDH, HPRT1 and RPLP0) was tested in ASCs cultured under standard protocol after inflammatory priming or starvation. Gene expression data were computed with four different applets able to rank genes depending on their stability in either single or combined conditions. The obtained final ranking suggests that for each treatment, a specific HKG is needed, and that starvation is the condition with the stronger effect on HKGs’ stability and, therefore, reliability. The normalization effect of proper HKGs’ use was then validated on three genes involved in OA and whose product is released by ASCs. Overall, data presented herein confirm that the choice of the best HKG has to be carefully considered and that each specific condition has to be tested to identify the most reliable candidate.

Published

2024

27. Role of the endoplasmic reticulum in mechanisms of aging and formation of senescent cells

Author

Lev Salnikov

Subjects

Aging, Endoplasmic reticulum, Ontogenesis, Housekeeping genes, Integrative genes, Senescent cells, Medicine

Abstract

The role of the endoplasmic reticulum (ER) in aging processes has not attracted much attention of researchers, while this structure plays one of the central roles in the processes of intracellular synthesis. Summarizing the data presented in this review, we can conclude that the number of polysomes is directly related to the production of proteins required by the cell. In turn, polysomes responsible for the production of specialized proteins are associated with the ER of highly differentiated cells. At the same time, proteins necessary for the functioning of cellular infrastructure are translated on free polysomes, which are not associated with the ER. During aging, an increase in the quantity or surface area of ER was also observed in cells, especially in senescent cells. Summarizing these data we can conclude that cell aging is directly related to changes in their ER, which lead to inhibition of the production of proteins necessary for the operation of cellular infrastructure. Therefore, it is possible to distinguish two targets for reducing age-related processes. These should be actions aimed at changing the ratio between ER-bound and free polysomes in favor of the last ones. The second goal is to regulate the amount of ER by enhancing membrane exchange in the cell. Together, these effects will be aimed at preserving the infrastructural base of cells, at least delaying their age-related degradation. As research progresses, unraveling the complex interplay between intracellular membranes and aging holds great promise for developing novel therapeutic strategies to combat age-related diseases and promote longevity.

Published

2024

28. Selection of suitable reference genes in Paulownia fortunei (Seem.) Hemsl. under different tissues and abiotic stresses for qPCR normalization

Author

Jiang Su, Kanghua Xian, Chuanming Fu, Jinxiang He, Baojun Liu, and Ningzhen Huang

Subjects

drought treatment, heavy metal, housekeeping genes, qrt-pcr, salinity treatment, Plant culture, SB1-1110

Abstract

By choosing appropriate candidate reference genes (CRGs) and standardizing qPCR data, more accurate experimental data can be obtained. Herein, the expression stability of alpha-tubulin1 (TUA1), beta-tubulin (TUB), beta-tubulin 1 (TUB1), beta-tubulin 5 (TUB5), actin 1 (ACT1), actin 97 (ACT97), molecular chaperone dnaj (DNAJ), adenine phosphoribosyl transferase (APT), and histone H4 (HIS4) genes from Paulownia fortunei (Seem.) Hemsl. under different experimental conditions (different tissues, drought, salinity, Cd, and Cr treatments) was assessed with four statistical tools: RefFinder, BestKeeper, NormFinder, and geNorm. Notably, TUA1 and TUB5 were identified as CRGs for different tissues, ACT97 and TUB1 for drought treatment, ACT97 and APT for salinity treatment, TUB1 and ACT97 for Cd treatment, and DNAJ, TUB1 and TUB5 for Cr treatment. Furthermore, the results of "total" group, V4/V5 > 0.15 and V5/V6 < 0.15 revealed that the CRGs or gene combinations, which could meet all the test conditions, were not easy to identify. To further verify the reliability of CRGs, the expression levels of paulownia fortunei cellulose synthase A catalytic subunit2 (PfCesA2) and paulownia fortunei glutathione reductase (GR) genes were analysed. The expression patterns were different when the unstable CRGs were used for normalization compared to when the stable CRGs and combination were used for normalization. This study will lay a foundation for study on the expression levels of key genes from P. fortunei seedlings.

Published

2023

29. Morphological and Phylogenetic Characterization of Whip Smut on Commercial Sugarcane Cultivars and Assessing the Resistance to Sporisorium scitamineum

Author

Amal Fazliarab, Reza Farokhinezhad, Mehdi Mehrabi-Koushki, Khosro Mehdikhanlou, and Koroush Taherkhani

Subjects

disease management, genetic diversity, housekeeping genes, whip smut, Genetics, QH426-470

Abstract

Whip smut, which is caused by Sporisorium scitamineum, is an important disease in areas where sugarcane is cultivated in Iran, particularly in the Khuzestan province. The pathogen significantly reduces sugarcane yield, and the use of resistant cultivars is the most cost-effective strategy for managing the disease. The present study characterized the S. scitamineum strains collected from five commercial sugarcane cultivars (CP69-1062, CP57-614, CP48-103, SP70-1143, and NCo310) based on their morphological and phylogenetic features. The sporidial cultures of the strains appeared in two growth forms: cottony colony and yeast-like. All strains were found to be identical based on the DNA sequences of ITS, COX3, GAPDH, and EF1α regions, and revealed that all strains were identical (100%) to the reference strain of S. scitamineum. The disease incidence of the cultivars varied from 5 to 43% during two consecutive years. Statistical analysis of the growth rates of the strains indicated significant differences. Combined analysis of variance (ANOVA) suggested that the effects of year, strain, cultivar, and the interaction effect of strain ´ cultivar were significant at a 1% probability level. Our results suggest that IRK310 was the most virulent among all cultivars, with different pathogenicity percentages, while the strain IRK70 had the lowest level of virulence among all strains. Among the tested cultivars, SP70-1143 and CP57-614 showed high resistance to smut. In this research, teliospore populations of whip smut were identified, and disease reactions of the cultivars were assayed. Screening and selecting smut-resistant cultivars can help reduce disease damage in cultivated areas and can serve as a basis for further research on plant disease management.

Published

2023

30. Housekeeping Gene Stability in Adipose Mesenchymal Stromal Cells Cultivated in Serum/Xeno-Free Media for Osteoarthritis.

Author

Ragni, Enrico, Piccolo, Simona, De Luca, Paola, Taiana, Michela, Grieco, Giulio, and de Girolamo, Laura

Subjects

*STROMAL cells, *ADIPOSE tissue physiology, *HOUSEKEEPING, *CURRENT good manufacturing practices, *OSTEOARTHRITIS, *CONSERVATIVE treatment

Abstract

Among the available therapeutics for the conservative treatment of osteoarthritis (OA), mesenchymal stromal cells (MSCs)-based products appear to be the most promising. Alongside minimally manipulated cell-based orthobiologics, where MSCs are the engine of the bioactive properties, cell expansion under good manufacturing practice (GMP) settings is actively studied to obtain clinical-grade pure populations able to concentrate the biological activity. One of the main characteristics of GMP protocols is the use of clinical-grade reagents, including the recently released serum-free/xeno-free (SFM/XFM) synthetic media, which differ significantly from the traditional reagents like those based on fetal bovine serum (FBS). As SFM/XFM are still poorly characterized, a main lack is the notion of reliable housekeeping genes (HKGs) for molecular studies, either standalone or in combination with standard conditions. Indeed, the aim of this work was to test the stability of five commonly used HKGs (ACTB, EF1A, GAPDH, RPLP0, and TBP) in adipose-derived MSCs (ASCs) cultivated in two commercially available SFM/XFM and to compare outcomes with those obtained in FBS. Four different applets widely recognized by the scientific community (NormFinder, geNorm, comparative ΔCt method, and BestKeeper) were used and data were merged to obtain a final stability order. The analysis showed that cells cultured in both synthetic media had a similar ranking for HKGs stability (GAPDH being best), albeit divergent from FBS expanded products (EF1A at top). Moreover, it was possible to identify specific HKGs for side by side studies, with EF1A/TBP being the most reliable normalizers for single SFM/XFM vs. FBS cultured cells and TBP the best one for a comprehensive analysis of all samples. In addition, stability of HKGs was donor-dependent. The normalization effect on selected genes coding for factors known to be involved in OA pathology, and whose amount should be carefully considered for the selection of the most appropriate MSC-based treatment, showed how HKGs choice might affect the perceived amount for the different media or donor. Overall, this work confirms the impact of SFM/XFM conditions on HKGs stability performance, which resulted similarly for both synthetic media analyzed in the study. [ABSTRACT FROM AUTHOR]

Published

2024

31. Selection and validation of optimal reference genes for RT-qPCR analyses in Aphidoletes aphidimyza Rondani (Diptera: Cecidomyiidae).

Author

Xiu-Xian Shen, Guo-Qiang Zhang, Yu-Xin Zhao, Xiao-Xiao Zhu, Xiao-Fei Yu, Mao-Fa Yang, and Feng Zhang

Subjects

MOLECULAR biology, GALL midges, CHEMOSENSORY proteins, GENE expression, AGRICULTURE

Abstract

Aphidoletes aphidimyza is a predator that is an important biological agent used to control agricultural and forestry aphids. Although many studies have investigated its biological and ecological characteristics, few molecular studies have been reported. The current study was performed to identify suitable reference genes to facilitate future gene expression and function analyses via quantitative reverse transcription PCR. Eight reference genes glyceraldehyde-3-phosphate dehydrogenase (GAPDH), RPS13, RPL8, RPS3, α-Tub, β-actin, RPL32, and elongation factor 1 alpha (EF1-α) were selected. Their expression levels were determined under four different experimental conditions (developmental stages, adult tissues, sugar treatment, and starvation treatment) using qRT-PCR technology. The stability was evaluated with five methods (Ct value, geNorm, NormFinder, BestKeeper, and RefFinder). The results showed that GAPDH, RPL32, and EF1-α were ranked as the best reference gene combinations for measuring gene expression levels among different developing stages and in various starvation treatments. RPL8 and RPS3 were recommended to normalize the gene expression levels among different adult tissues. RPL32, β-actin, and EF1-α were recommended sugar-feeding conditions. To validate the utility of the selected reference pair, RPL8, and RPS3, we estimated the tissue-biased expression level of a chemosensory protein gene (AaphCSP1). As expected, AaphCSP1 is highly expressed in the antennae and lowly expressed in the abdomen. These findings will lay the foundation for future research on the molecular physiology and biochemistry of A. aphidimyza. [ABSTRACT FROM AUTHOR]

Published

2023

32. Study of mRNA expression levels in steady state Trypanosoma evansi for plausible selection of housekeeping and drug target genes

Author

Gupta, Snehil, Vohra, Sukhdeep, and Kumar, Rajender

Published

2023

33. Reference genes for gene expression profiling in mouse models of Listeria monocytogenes infection

Author

Lethicia Souza Tavares, Roberta Lane Oliveira-Silva, Marcelo Tigre Moura, Jéssica Barboza da Silva, Ana Maria Benko-Iseppon, and José Vitor Lima-Filho

Subjects

cytokine, housekeeping genes, immune response, internal control genes, listeriosis, macrophages, Biology (General), QH301-705.5

Abstract

RT-qPCR dissects transcription-based processes but requires reference genes (RGs) for data normalization. This study prospected RGs for mouse macrophages (pMØ) and spleen infected with Listeria monocytogenes. The pMØ were infected in vitro with L. monocytogenes or vehicle for 4 h. Mice were injected with L. monocytogenes (or vehicle) and euthanized 24 h post-injection. The RGs came from a multispecies primer set, from the literature or designed here. The RG ranking relied on GeNorm, NormFinder, BestKeeper, Delta-CT and RefFinder. B2m-H3f3a-Ppia were the most stable RGs for pMØ, albeit RG indexes fine-tuned estimations of cytokine relative expression. Actβ-Ubc-Ppia were the best RGs for spleen but modestly impacted the cytokine relative expression. Hence, mouse models of L. monocytogenes require context-specific RGs for RT-qPCR, thus reinforcing its paramount contribution to accurate gene expression profiling.

Published

2023

34. The MADF-BESS Protein CP60 Is Recruited to Insulators via CP190 and Has Redundant Functions in Drosophila.

Author

Melnikova, Larisa, Molodina, Varvara, Babosha, Valentin, Kostyuchenko, Margarita, Georgiev, Pavel, and Golovnin, Anton

Subjects

*DROSOPHILA, *TRANSCRIPTION factors, *GENE expression, *GENETIC transcription regulation, *PROTEINS

Abstract

Drosophila CP190 and CP60 are transcription factors that are associated with centrosomes during mitosis. CP190 is an essential transcription factor and preferentially binds to housekeeping gene promoters and insulators through interactions with architectural proteins, including Su(Hw) and dCTCF. CP60 belongs to a family of transcription factors that contain the N-terminal MADF domain and the C-terminal BESS domain, which is characterized by the ability to homodimerize. In this study, we show that the conserved CP60 region adjacent to MADF is responsible for interacting with CP190. In contrast to the well-characterized MADF-BESS transcriptional activator Adf-1, CP60 is recruited to most chromatin sites through its interaction with CP190, and the MADF domain is likely involved in protein–protein interactions but not in DNA binding. The deletion of the Map60 gene showed that CP60 is not an essential protein, despite the strong and ubiquitous expression of CP60 at all stages of Drosophila development. Although CP60 is a stable component of the Su(Hw) insulator complex, the inactivation of CP60 does not affect the enhancer-blocking activity of the Su(Hw)-dependent gypsy insulator. Overall, our results indicate that CP60 has an important but redundant function in transcriptional regulation as a partner of the CP190 protein. [ABSTRACT FROM AUTHOR]

Published

2023

35. Different Protein Groups Involved in Transcription Regulation in Development and Housekeeping Genes in Drosophila.

Author

Zhimulev, I. F., Vatolina, T. Yu., Pokholkova, G. V., Antonenko, O. V., and Maltseva, M. V.

Subjects

*GENETIC transcription regulation, *DROSOPHILA, *HOUSEKEEPING, *GENES, *CHROMOSOME banding

Abstract

Antibodies to histone modifications and an insulator protein involved in the processes of transcription initiation and elongation are mapped in Drosophila polytene chromosomes. The CHRIZ protein (chromatin insulator) and H3K36me3 histone modification (RNA elongation) are detected only in the localization of housekeeping genes (interbands and gray bands of polytene chromosomes) and never in the regions of developmental genes (black bands and large puffs arising from them). Antibodies to H3S10P histone modification, which is associated with the initial elongation of the RNA strand during transcription, are found exclusively in small puffs, but not in housekeeping gene localization sites or large ecdysone-induced puffs, where housekeeping genes are localized. Antibodies to H4R3me2 histone modification (a co-repressor of the ecdysone receptor) are detected only in large ecdysone-induced puffs. [ABSTRACT FROM AUTHOR]

Published

2023

36. The outstanding diversity of rhizobia microsymbionts of common bean (Phaseolus vulgaris L.) in Mato Grosso do Sul, central-western Brazil, revealing new Rhizobium species.

Author

Moura, Fernanda Terezinha, Helene, Luisa Caroline Ferraz, Ribeiro, Renan Augusto, Nogueira, Marco Antonio, and Hungria, Mariangela

Abstract

Common bean is considered a legume of great socioeconomic importance, capable of establishing symbioses with a wide variety of rhizobial species. However, the legume has also been recognized for its low efficiency in fixing atmospheric nitrogen. Brazil is a hotspot of biodiversity, and in a previous study, we identified 13 strains isolated from common bean (Phaseolus vulgaris) nodules in three biomes of Mato Grosso do Sul state, central-western Brazil, that might represent new phylogenetic groups, deserving further polyphasic characterization. The phylogenetic tree of the 16S rRNA gene split the 13 strains into two large clades, seven in the R. etli and six in the R. tropici clade. The MLSA with four housekeeping genes (glnII, gyrB, recA, and rpoA) confirmed the phylogenetic allocation. Genomic comparisons indicated eight strains in five putative new species and the remaining five as R. phaseoli. The average nucleotide identity (ANI) and digital DNA–DNA hybridization (dDDH) comparing the putative new species and the closest neighbors ranged from 81.84 to 92.50% and 24.0 to 50.7%, respectively. Other phenotypic, genotypic, and symbiotic features were evaluated. Interestingly, some strains of both R. etli and R. tropici clades lost their nodulation capacity. The data support the description of the new species Rhizobium cerradonense sp. nov. (CNPSo 3464T), Rhizobium atlanticum sp. nov. (CNPSo 3490T), Rhizobium aureum sp. nov. (CNPSo 3968T), Rhizobium pantanalense sp. nov. (CNPSo 4039T), and Rhizobium centroccidentale sp. nov. (CNPSo 4062T). [ABSTRACT FROM AUTHOR]

Published

2023

37. Evaluation of reference genes for quantitative analysis of gene expression in Lippia alba under abiotic stress.

Author

Nascimento, Laís Stehling de Queiroz, Lopes, Juliana Mainenti Leal, de Matos, Elyabe Monteiro, Souza, Vinicius Carius, Batista, Diego Silva, Santos, Marcelo de Oliveira, Otoni, Wagner Campos, and Viccini, Lyderson Facio

Abstract

Lippia alba (Mill.) N.E. Brown (Verbenaceae) is a medicinal plant of commercial interest because it is a source of essential oils, such as citral and linalool. Abiotic stress can modulate biosynthetic pathways and regulate the production of secondary metabolites found in essential oils. RT-qPCR is a useful tool for investigating the expression of biosynthetic genes and select cultivars with improved essential oil composition. However, RT-qPCR requires normalization to a stable reference genes, appropriate for each experimental condition. Here, we describe the evaluation of reference genes for RT-qPCR analysis in L. alba. Six constitutive genes (NADH, CIT, G6i, TUB, RNApol, and ELONG) were analyzed using BestKeeper, GeNorm, NormFinder, and RefFinder software. TUB emerged as the most stable gene under osmotic stress; whereas NADH was most stable under saline, wounding, cold, and exogenous abscisic acid and salicylic acid stress. Therefore, TUB and NADH are recommended for use as reference genes in expression studies involving L. alba. Key message: Experimental conditions affect the expression of reference genes. NADH is the most stable gene under saline, exogenous hormones, wounding, and cold stress; whereas TUB is most stable under osmotic stress. [ABSTRACT FROM AUTHOR]

Published

2023

38. Deciphering the sex bias in housekeeping gene expression in adipose tissue: a comprehensive meta-analysis of transcriptomic studies

Author

Maria Guaita-Cespedes, Rubén Grillo-Risco, Marta R. Hidalgo, Sonia Fernández-Veledo, Deborah Jane Burks, María de la Iglesia-Vayá, Amparo Galán, and Francisco Garcia-Garcia

Subjects

Housekeeping genes, Meta-analysis, Transcriptomics, Sex bias, Adipose tissue, Medicine, Physiology, QP1-981

Abstract

Abstract Background As the housekeeping genes (HKG) generally involved in maintaining essential cell functions are typically assumed to exhibit constant expression levels across cell types, they are commonly employed as internal controls in gene expression studies. Nevertheless, HKG may vary gene expression profile according to different variables introducing systematic errors into experimental results. Sex bias can indeed affect expression display, however, up to date, sex has not been typically considered as a biological variable. Methods In this study, we evaluate the expression profiles of six classical housekeeping genes (four metabolic: GAPDH, HPRT, PPIA, and UBC, and two ribosomal: 18S and RPL19) to determine expression stability in adipose tissues (AT) of Homo sapiens and Mus musculus and check sex bias and their overall suitability as internal controls. We also assess the expression stability of all genes included in distinct whole-transcriptome microarrays available from the Gene Expression Omnibus database to identify sex-unbiased housekeeping genes (suHKG) suitable for use as internal controls. We perform a novel computational strategy based on meta-analysis techniques to identify any sexual dimorphisms in mRNA expression stability in AT and to properly validate potential candidates. Results Just above half of the considered studies informed properly about the sex of the human samples, however, not enough female mouse samples were found to be included in this analysis. We found differences in the HKG expression stability in humans between female and male samples, with females presenting greater instability. We propose a suHKG signature including experimentally validated classical HKG like PPIA and RPL19 and novel potential markers for human AT and discarding others like the extensively used 18S gene due to a sex-based variability display in adipose tissue. Orthologs have also been assayed and proposed for mouse WAT suHKG signature. All results generated during this study are readily available by accessing an open web resource ( https://bioinfo.cipf.es/metafun-HKG ) for consultation and reuse in further studies. Conclusions This sex-based research proves that certain classical housekeeping genes fail to function adequately as controls when analyzing human adipose tissue considering sex as a variable. We confirm RPL19 and PPIA suitability as sex-unbiased human and mouse housekeeping genes derived from sex-specific expression profiles, and propose new ones such as RPS8 and UBB.

Published

2023

39. Evaluation of reference genes for transcript analyses in Komagataella phaffii (Pichia pastoris)

Author

Mihail Besleaga, Gabriel A. Vignolle, Julian Kopp, Oliver Spadiut, Robert L. Mach, Astrid R. Mach-Aigner, and Christian Zimmermann

Subjects

Komagataella phaffii, Pichia pastoris, RT-qPCR, Relative transcript analysis, Transcriptomics, Housekeeping genes, Biotechnology, TP248.13-248.65

Abstract

Abstract Background The yeast Komagataella phaffii (Pichia pastoris) is routinely used for heterologous protein expression and is suggested as a model organism for yeast. Despite its importance and application potential, no reference gene for transcript analysis via RT-qPCR assays has been evaluated to date. In this study, we searched publicly available RNASeq data for stably expressed genes to find potential reference genes for relative transcript analysis by RT-qPCR in K. phaffii. To evaluate the applicability of these genes, we used a diverse set of samples from three different strains and a broad range of cultivation conditions. The transcript levels of 9 genes were measured and compared using commonly applied bioinformatic tools. Results We could demonstrate that the often-used reference gene ACT1 is not very stably expressed and could identify two genes with outstandingly low transcript level fluctuations. Consequently, we suggest the two genes, RSC1, and TAF10 to be simultaneously used as reference genes in transcript analyses by RT-qPCR in K. phaffii in future RT-qPCR assays. Conclusion The usage of ACT1 as a reference gene in RT-qPCR analysis might lead to distorted results due to the instability of its transcript levels. In this study, we evaluated the transcript levels of several genes and found RSC1 and TAF10 to be extremely stable. Using these genes holds the promise for reliable RT-qPCR results.

Published

2023

40. A multi locus sequence analysis scheme for phylogeny of the Bacillus subtilis species complex and its advantages over 16S rRNA genes

Author

Dao Nu Dieu Hong, Trang Hoang Long, Nguyen Thi Thuy Tien, Dinh Anh Hoa, Tran Thi Phan, and Le Thi Huynh Tram

Subjects

a multi locus sequence analysis (mlsa approach), bacillus subtilis, housekeeping genes, 16s rrna, Biotechnology, TP248.13-248.65

Abstract

A multi locus sequence analysis (MLSA approach) was studied on the Bacillus genus, or the Bacillus subtilis species complex for specific, including 08 strains from four species (B. subtilis, B. pumilus, B. licheniformis and B. amyloliquefaciens) were provided by Biotechnology Center of Ho Chi Minh City. The research was based on sequences of 16S rRNA genes, the concatenation of five protein-coding housekeeping genes: glpF, pta, purH, pycA, and rpoD. After PCR amplification and sequencing the phylogenetic tree of 16S rRNA sequences, concatenate sequences (as well as the phylogenetic tree of each housekeeping gene) are constructed for comparison and discussion. The aim of this study is reach for better resolution and differentiation of strains and species within the B. subtilis species and to determine whether MLSA scheme show advantages in 16S rRNA gene-based studies.

Published

2022

41. Morphological and Phylogenetic Characterization of Whip Smut on Commercial Sugarcane Cultivars and Assessing the Resistance to Sporisorium scitamineum.

Author

Fazliarab, Amal, Farokhinejad, Reza, Mehrabi-Koushki, Mehdi, Khanlou, Khosro Mehdi, and Taherkhan, Kourosh

Subjects

SUGARCANE harvesting, PHYLOGENY, PLANT diseases, GENETIC variation, ANALYSIS of variance

Abstract

Whip smut, which is caused by Sporisorium scitamineum, is an important disease in areas where sugarcane is cultivated in Iran, particularly in the Khuzestan province. The pathogen significantly reduces sugarcane yield, and the use of resistant cultivars is the most cost-effective strategy for managing the disease. The present study characterized the S. scitamineum strains collected from five commercial sugarcane cultivars (CP69-1062, CP57-614, CP48-103, SP70-1143, and NCo310) based on their morphological and phylogenetic features. The sporidial cultures of the strains appeared in two growth forms: cottony colony and yeast-like. All strains were found to be identical based on the DNA sequences of ITS, COX3, GAPDH, and EF1α regions, and revealed that all strains were identical (100%) to the reference strain of S. scitamineum. The disease incidence of the cultivars varied from 5 to 43% during two consecutive years. Statistical analysis of the growth rates of the strains indicated significant differences. Combined analysis of variance (ANOVA) suggested that the effects of year, strain, cultivar, and the interaction effect of strain x cultivar were significant at a 1% probability level. Our results suggest that IRK310 was the most virulent among all cultivars, with different pathogenicity percentages, while the strain IRK70 had the lowest level of virulence among all strains. Among the tested cultivars, SP70-1143 and CP57-614 showed high resistance to smut. In this research, teliospore populations of whip smut were identified, and disease reactions of the cultivars were assayed. Screening and selecting smut-resistant cultivars can help reduce disease damage in cultivated areas and can serve as a basis for further research on plant disease management. [ABSTRACT FROM AUTHOR]

Published

2023

42. اولین گزارش باکتری Pantoea dispersa در ایران.

Author

حسنا الوندى and و سید محسن تقوی

Subjects

WHEAT, CORN, LEAF spots, PATHOGENIC bacteria, MILLETS

Abstract

Corn (Zea mays) is from the cereal category and the large wheat family; it is the third crop after wheat and rice cultivated areas worldwide. This research aims to investigate the detection and identification of the pathogenic bacterium Pantoea dispersa in Iran using biochemical and molecular identification methods and the host range of this bacterial species. For this purpose, in two consecutive years, sampling was done from the corn fields of different provinces of Iran, which have symptoms such as leaf spots and wilting. Standard plant bacteriology methods were used to isolate bacteria with the mentioned symptoms, and isolates were identified using biochemical characteristics and primers related to housekeeping genes. In the investigation of pathogenicity and host range of 20 bacterial isolates obtained from different corn fields, six isolates were identified as P. dispersa. This is the first report of the presence of the bacterium in Iran. In examining the host range of the mentioned isolates millet and sourghum are introduced as new hosts of this species in Iran. [ABSTRACT FROM AUTHOR]

Published

2023

43. The Interplay Between the Transcriptomics and Proteomics Profiles

Author

Teibo, John Oluwafemi, Silvestrini, Virgínia Campos, Vargas, Alessandra P., Lanfredi, Guilherme Pauperio, Faça, Vítor Marcel, and Passos, Geraldo A., editor

Published

2022

44. Expression of housekeeping genes varies depending on mevalonate pathway inhibition in cancer cells

Author

Nanami Irie, Katsuhiko Warita, Jiro Tashiro, Yaxuan Zhou, Takuro Ishikawa, Zoltán N. Oltvai, and Tomoko Warita

Subjects

Mevalonate pathway, Cancer cells, Statins, Housekeeping genes, RT-qPCR, Optimal internal reference genes, Science (General), Q1-390, Social sciences (General), H1-99

Abstract

Statins have anticancer effects and may be used as anticancer agents via drug repositioning. In reverse transcription-quantitative polymerase chain reaction (RT-qPCR) assays, the internal reference gene must not be affected by any experimental conditions. As statins exert a wide range of effects on cells by inhibiting the mevalonate pathway, it is possible that statin treatment might alter the expression of housekeeping genes used as internal reference genes, thereby misleading the assessment of obtained gene expression data. Here, we evaluated the expression stability of internal reference genes in atorvastatin-treated cancer cell lines. We treated both statin-sensitive and statin-resistant cancer cell lines with atorvastatin at seven different concentrations and performed RT-qPCR on 15 housekeeping genes whose expression stability was then assessed using five different algorithms. In both statin-sensitive and statin-resistant cancer cell lines, atorvastatin affected the expression of certain internal reference genes in a dose-dependent and cancer cell line-dependent manner; therefore, caution should be exercised when comparing target gene expression between cells. Our findings emphasize the importance of the validation of internal reference genes in gene expression analyses in drug treatment-based cancer research.

Published

2023

45. Deciphering the sex bias in housekeeping gene expression in adipose tissue: a comprehensive meta-analysis of transcriptomic studies.

Author

Guaita-Cespedes, Maria, Grillo-Risco, Rubén, Hidalgo, Marta R., Fernández-Veledo, Sonia, Burks, Deborah Jane, de la Iglesia-Vayá, María, Galán, Amparo, and Garcia-Garcia, Francisco

Subjects

*SEXISM, *GENE expression, *GENE expression profiling, *ADIPOSE tissues, *HOUSEKEEPING, *TRANSCRIPTOMES

Abstract

Background: As the housekeeping genes (HKG) generally involved in maintaining essential cell functions are typically assumed to exhibit constant expression levels across cell types, they are commonly employed as internal controls in gene expression studies. Nevertheless, HKG may vary gene expression profile according to different variables introducing systematic errors into experimental results. Sex bias can indeed affect expression display, however, up to date, sex has not been typically considered as a biological variable. Methods: In this study, we evaluate the expression profiles of six classical housekeeping genes (four metabolic: GAPDH, HPRT, PPIA, and UBC, and two ribosomal: 18S and RPL19) to determine expression stability in adipose tissues (AT) of Homo sapiens and Mus musculus and check sex bias and their overall suitability as internal controls. We also assess the expression stability of all genes included in distinct whole-transcriptome microarrays available from the Gene Expression Omnibus database to identify sex-unbiased housekeeping genes (suHKG) suitable for use as internal controls. We perform a novel computational strategy based on meta-analysis techniques to identify any sexual dimorphisms in mRNA expression stability in AT and to properly validate potential candidates. Results: Just above half of the considered studies informed properly about the sex of the human samples, however, not enough female mouse samples were found to be included in this analysis. We found differences in the HKG expression stability in humans between female and male samples, with females presenting greater instability. We propose a suHKG signature including experimentally validated classical HKG like PPIA and RPL19 and novel potential markers for human AT and discarding others like the extensively used 18S gene due to a sex-based variability display in adipose tissue. Orthologs have also been assayed and proposed for mouse WAT suHKG signature. All results generated during this study are readily available by accessing an open web resource (https://bioinfo.cipf.es/metafun-HKG) for consultation and reuse in further studies. Conclusions: This sex-based research proves that certain classical housekeeping genes fail to function adequately as controls when analyzing human adipose tissue considering sex as a variable. We confirm RPL19 and PPIA suitability as sex-unbiased human and mouse housekeeping genes derived from sex-specific expression profiles, and propose new ones such as RPS8 and UBB. Plain English Summary: Housekeeping genes (HKG) are involved in the maintenance of essential cellular functions. They usually present constant expression levels and are relevant because of their usefulness as internal controls in gene expression studies. However, HKG can vary the gene expression profile depending on different variables such as sex, introducing errors in the experimental results. In this study, we have performed an exhaustive systematic review and applied a massive analysis of expression data to check which HKG presents this bias and which do not. The results confirm that certain classical HKG do not perform adequately as controls when analyzing human adipose tissue considering sex as a variable. We further confirm the suitability of RPL19 and PPIA as human and mouse HKG without sex bias derived from sex-specific expression profiles, and propose new ones such as RPS8 and UBB. These results will be of great use in upcoming studies where expression data need to be normalized without the inclusion of sex bias. Highlights: A computational strategy based on massive data analysis revealed that an accurate experimental design for adipose tissue requires the adequate selection of a sex-unbiased housekeeping genes (HKG). The extensively used 18S gene displays sex-based variability in adipose tissue, although PPIA and RPL19 do not, and hence, represent robust HKG. New sex-unbiased human and mouse candidate HKG: RPS8 and UBB. metafun-HKG (https://bioinfo.cipf.es/metafun-HKG): a freely available web tool to allow users to review stable expression levels of candidate HKG along the large volume of FAIR data. [ABSTRACT FROM AUTHOR]

Published

2023

46. Reference genes for quantitative Arabidopsis single molecule RNA fluorescence in situ hybridization.

Author

Duncan, Susan, Johansson, Hans E, and Ding, Yiliang

Subjects

*SINGLE molecules, *FLUORESCENCE in situ hybridization, *REGULATOR genes, *RNA, *ARABIDOPSIS, *MOLECULAR probes

Abstract

Subcellular mRNA quantities and spatial distributions are fundamental for driving gene regulatory programmes. Single molecule RNA fluorescence in situ hybridization (smFISH) uses fluorescent probes to label individual mRNA molecules, thereby facilitating both localization and quantitative studies. Validated reference mRNAs function as positive controls and are required for calibration. Here we present selection criteria for the first set of Arabidopsis smFISH reference genes. Following sequence and transcript data assessments, four mRNA probe sets were selected for imaging. Transcript counts per cell, correlations with cell size, and corrected fluorescence intensities were all calculated for comparison. In addition to validating reference probe sets, we present sample preparation steps that can retain green fluorescent protein fluorescence, thereby providing a method for simultaneous RNA and protein detection. In summary, our reference gene analyses, modified protocol, and simplified quantification method together provide a firm foundation for future quantitative single molecule RNA studies in Arabidopsis root apical meristem cells. [ABSTRACT FROM AUTHOR]

Published

2023

47. Development of N.K. Koltsov's Idea about Genetic Organization of Interbands in Drosophila melanogaster Polytene Chromosomes.

Author

Zhimulev, I. F., Vatolina, T. Yu., Levitsky, V. G., Kolesnikova, T. D., and Tsukanov, A. V.

Subjects

*DROSOPHILA melanogaster, *CHROMOSOMES, *CELL physiology, *DROSOPHILA, *GENE ontology, *DROSOPHILIDAE

Abstract

The organization of promoters of developmental gene promoters and promoter of genes necessary for general cellular functions—the "housekeeping" of the cell in the complete genome of Drosophila melanogaster—were studied here for the first time. Using bioinformatic methods, it has been shown that the genes whose promoters are located in the interbands of polytene chromosomes are enriched in functions associated with general cellular processes, while the rest of the genes (approximately half of the Drosophila genome) are associated with highly specialized processes occurring during development. In the promoter zone of the housekeeping genes, four specific motifs were found that can be present in different genes individually or in various combinations. A significant part of interband promoters do not contain identified motifs. The analysis carried out using Gene Ontology showed that certain groups of interband genes containing one motif in promoters or their combinations are characterized by the performance of certain functions. [ABSTRACT FROM AUTHOR]

Published

2023

48. Conservative Protein RCC1 Is a New Component of Black Bands of Drosophilamelanogaster Polytene Chromosomes.

Author

Zykova, T. Yu., Maltseva, M. V., Demakov, S. A., Pokholkova, G. V., Veryaskina, Yu. A., Lavrik, O. I., Kolesnikova, T. D., and Zhimulev, I. F.

Subjects

*CHROMOSOMES, *AMINO acid sequence, *NUCLEAR proteins, *CHROMOSOME banding, *CARRIER proteins

Abstract

Previously, the RCC1 gene (Regulator of Chromosome Condensation 1), which is considered a regulator of chromosome condensation in the cell cycle, was characterized. This gene encodes a nuclear protein whose amino acid sequence is highly conserved among all eukaryotes and consists of seven repeating units. The authors have shown that all the most prominent black bands of polytene chromosomes (260 bands) and the chromocenter bind antibodies to this protein. Antibodies to the xenopus RCC1 protein specifically bind to the Drosophila and human RCC1 protein, while the relative amount of the RCC1 protein increases in Drosophila lines with under-replication suppression compared to the wild type. [ABSTRACT FROM AUTHOR]

Published

2023

49. Insights into Early Ontogenesis of Salmo salar : RNA Extraction, Housekeeping Gene Validation and Transcriptional Expression of Important Primordial Germ Cell and Sex-Determination Genes.

Author

Bhat, Irfan Ahmad, Dubiel, Milena Malgorzata, Rodriguez, Eduardo, and Jónsson, Zophonías Oddur

Subjects

*GENE expression, *ATLANTIC salmon, *GERM cells, *SEX determination, *ONTOGENY, *COMPREHENSION in children

Abstract

Simple Summary: The development of primordial germ cells (PGCs) and sex determination (SD) is governed by a complex interplay of genes that can be targeted to hinder sexual development in fish. Obtaining high-quality ribonucleic acid (RNA) from Atlantic salmon embryos, especially after fertilization, can be extremely challenging due to the presence of a substantial amount of yolk. The objective of this research was to extract high-quality RNA from developing salmon embryos for use in downstream applications. The study also aimed to validate different housekeeping genes (HKGs) for a quantitative polymerase chain reaction (qPCR)-based assessment of PGC and SD genes during developmental stages in salmon. We isolated RNA from the developing embryos, and we present the validation of HKGs as well as the mRNA expression levels of important PGC and SD genes during the fertilization to hatching stage. The findings of this study could prove beneficial for researchers seeking to extract high-quality RNA from salmonids. Moreover, the transcript results may offer insights not only into the function of transcripts at specific developmental stages but also in identifying the stage with the highest expression levels, during which treatment to disrupt the function of the transcripts and ultimately the growth of PGCs could be administered. The challenge in extracting high-quality RNA impedes the investigation of the transcriptome of developing salmonid embryos. Furthermore, the mRNA expression pattern of important PGC and SD genes during the initial embryonic development of Salmo salar is yet to be studied. So, in the present study, we aimed to isolate high-quality RNA from eggs and developing embryos to check vasa, dnd1, nanos3a, sdf1, gsdf, amh, cyp19a, dmrt1 and foxl2 expression by qPCR. Additionally, four HKGs (GAPDH, UB2L3, eEf1a and β-actin) were validated to select the best internal control for qPCR. High-quality RNA was extracted, which was confirmed by spectrophotometer, agarose gel electrophoresis and Agilent TapeStation analysis. UB2L3 was chosen as a reference gene because it exhibited lower intra- and inter-sample variation. vasa transcripts were expressed in all the developmental stages, while dnd1 was expressed only up to 40 d°C. Nanos3a was expressed in later stages and remained at its peak for a shorter period, while sdf1 showed an irregular pattern of mRNA expression. The mRNA expression levels of SD genes were observed to be upregulated during the later stages of development, prior to hatching. This study presents a straightforward methodology for isolating high-quality RNA from salmon eggs, and the resulting transcript profiles of significant PGC and SD genes in S. salar could aid in improving our comprehension of reproductive development in this commercially important species. [ABSTRACT FROM AUTHOR]

Published

2023

50. Multidrug resistance protein 1 silencing in osteosarcoma and chondrosarcoma cell lines.

Author

Freund, Sarah S., Bendtsen, Michael M., Safwat, Akmal, and Joergensen, Peter H.

Subjects

*P-glycoprotein, *CHONDROSARCOMA, *SMALL interfering RNA, *GENE expression, *CELL lines

Abstract

Background: The poor response of metastatic osteo- and chondrosarcomas to chemotherapy could be the result of multidrug resistance (MDR), which may be overcome through the use of small interfering RNA (siRNA). However, several methodologic questions remain unresolved. Aims: To test the toxicity of three commonly used siRNA transfection reagents and apply the least toxic reagent to investigate the siRNA-induced MDR1 mRNA knockdown. Methods: The toxicity of TransIT-TKO, Lipofectamine 2000, and X-tremeGENE siRNA transfection reagents was investigated on osteosarcoma (MG-63) and chondrosarcoma (SW1353) cell lines. The toxicity was measured at 4 and 24 hours using a MTT toxicity assay. The least toxic transfection reagent was applied to investigate the siRNA-induced MDR1 mRNA knockdown effect using qRT-PCR. Furthermore, five housekeeping genes were assessed in the BestKeeper software to obtain mRNA expression normalization. Results: Lipofectamine 2000 was the least toxic transfection reagent, reducing the cell viability only in chondrosarcoma 24 hours following exposure to the highest dose. In contrast, TransIT-TKO and X-tremeGENE transfection reagents displayed a significant reduction in cell viability in both chondrosarcoma after 4 hours and in osteosarcoma after 24 hours. Significant MDR1 mRNA silencing of over 80% was achieved in osteo- and chondrosarcoma using Lipofectamine at a final siRNA concentration of 25 nM. No significant dose response was observed in knockdown efficiency in either Lipofectamine or siRNA concentration. Conclusion: Lipofectamine 2000 was the least toxic transfection reagent in osteo- and chondrosarcoma. Successful siRNA-induced MDR1 mRNA silencing of over 80% was achieved. [ABSTRACT FROM AUTHOR]

Published

2023