Comparison of microRNA expression profiles in K562-cells-derived microvesicles and parental cells, and analysis of their roles in leukemia

Chen, Xiaomei; Xiong, Wei; Li, Huiyu

doi:10.3892/ol.2016.5308

Cited by 15 publications

(7 citation statements)

References 59 publications

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“…Pffafl estimated that a 10 fold increase in starting RNA/DNA copy numbers in RT‐ qPCR results in a 3.31 decrease in the Ct value . Furthermore, the selected miRNA sequences were reported to have different abundance levels in K562 , but the reported relative amount and absolute copy number varied a lot from one source to the other, for example some sources report equal elevation of miR‐103 and miR‐107 while other sources report a more than 40 fold elevation in miR‐103 over miR‐107 . Note that this discrepancy by no means indicates an error but highlights the variability in miRNA concentration even for the same cell line.…”

Section: Resultsmentioning

confidence: 99%

Isolation of enriched small RNA from cell‐lysate using on‐chip isotachophoresis

2019

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In spite of the growing interest in the roles and applications of small RNAs (sRNAs), sRNA isolation methods are inconsistent, tedious, and dependent on the starting number of cells. In this work, we employ ITP to isolate sRNAs from the cell‐lysate of K562 (chronic myelogenous leukemia) cells in a polydimethylsiloxane (PDMS) mesofluidic device. Our method specifically purifies sRNA of <60 nucleotides from lysate of a wide range of cell number spanning from 100 to 1 000 000 cells. We measured the amount of sRNA using the Agilent Bioanalyzer and further verified the extraction efficiency by reverse transcription quantitative PCR. Our method was shown to be more efficient in sRNA extraction than commercial sRNA isolation kits, especially when using smaller numbers of starting cells. Our assay presents a simple and rapid sRNA extraction method with 20 min assay time and no intermediate transfer steps.

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Section: Resultsmentioning

confidence: 99%

Isolation of enriched small RNA from cell‐lysate using on‐chip isotachophoresis

2019

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“…37 Moreover, it was demonstrated that miR-185 enhanced glucocorticoid sensitivity via suppressing the mTORC signaling pathway, 37 suggesting miR-185 as a potential target for diagnosis and reversion of glucocorticoid resistance. Chen et al 38 investigated specific variations of miRNA expression patterns in microvesicles (MVs) derived from CML K562 cells, and miR-185 was expressed both in MVs derived from K562 cells and in K562 cells. Whereas there was no data to illuminate the role of miR-185 in AML.…”

Section: Discussionmentioning

confidence: 99%

<p>Long Non-Coding RNA Taurine Upregulated Gene 1 Targets miR-185 to Regulate Cell Proliferation and Glycolysis in Acute Myeloid Leukemia Cells in vitro</p>

Zhang

Liu²,

Zhang

et al. 2020

OTT

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Background Acute myeloid leukemia (AML) is a group of malignant hematopoietic system diseases. Taurine-upregulated gene 1 (TUG1) is a long non-coding RNA that has been associated with human cancers, including AML. However, the role and molecular mechanisms of TUG1 in AML remains to be defined. Methods Expression of TUG1 and miR-185 was detected using RT-qPCR. Cell viability and apoptotic rate were measured by MTT assay and flow cytometry, respectively. Glycolysis was determined by commercial glucose and lactate assay kits and Western blot. The target binding between TUG1 and miR-185 was predicted on Starbase online database and confirmed by luciferase reporter assay and RNA immunoprecipitation. Results TUG1 was upregulated and miR-185 was downregulated in the peripheral blood mononuclear cells of AML specimens and cells (HL-60, KG-1, MOLM-14, and MOLM-13). Both TUG1 knockdown and miR-185 overexpression via transfection could suppress cell viability, glucose consumption, lactate production, and hexokinase 2 expression, but promote apoptotic rate in HL-60 and KG-1 cells. Notably, TUG1 functioned as a sponge of miR-185 by target binding. Moreover, downregulation of miR-185 could partially overturn the effect of TUG1 knockdown on cell proliferation and glycolysis in HL-60 and KG-1 cells. Conclusion Expression of TUG1 was upregulated in AML patients and cells, and its knockdown repressed cell proliferation and glycolysis in AML cells in vitro by targeting miR-185.

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“…Moreover, 20% of studied miRNAs were presented at higher levels in microvesicles than in cells of origin. In this research, an active and selective process of miRNA incorporation in microvesicles was hypothesized for the K562 cell line (39).…”

Section: Discussionmentioning

confidence: 99%

Expression Profiling of Circulating Microvesicles Reveals Intercellular Transmission of Oncogenic Pathways

Milani

Lana

Bresolin

et al. 2017

Molecular Cancer Research

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Circulating microvesicles have been described as important players in cell-to-cell communication carrying biological information under normal or pathologic condition. Microvesicles released by cancer cells may incorporate diverse biomolecules (e.g., active lipids, proteins, and RNA), which can be delivered and internalized by recipient cells, potentially altering the gene expression of recipient cells and eventually impacting disease progression. Leukemia in vitro model systems were used to investigate microvesicles as vehicles of protein-coding messages. Several leukemic cells (K562, LAMA-87, TOM-1, REH, and SHI-1), each carrying a specific chromosomal translocation, were analyzed. In the leukemic cells, these chromosomal translocations are transcribed into oncogenic fusion transcripts and the transfer of these transcripts was monitored from leukemic cells to microvesicles for each of the cell lines. Microarray gene expression profiling was performed to compare transcriptomes of K562-derived microvesicles and parental K562 cells. The data show that oncogenic BCR-ABL1 transcripts and mRNAs related to basic functions of leukemic cells were included in microvesicles. Further analysis of microvesicles cargo revealed a remarkable enrichment of transcripts related to cell membrane activity, cell surface receptors, and extracellular communication when compared with parental K562 cells. Finally, coculturing of healthy mesenchymal stem cells (MSC) with K562-derived microvesicles displayed the transfer of the oncogenic message, and confirmed the increase of target cell proliferation as a function of microvesicle dosage.Implications: This study provides novel insight into tumorderived microvesicles as carriers of oncogenic protein-coding messages that can potentially jeopardize cell-directed therapy, and spread to other compartments of the body. Mol Cancer Res; 15(6); 683-95. Ó2017 AACR.

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Comparison of microRNA expression profiles in K562-cells-derived microvesicles and parental cells, and analysis of their roles in leukemia

Cited by 15 publications

References 59 publications

Isolation of enriched small RNA from cell‐lysate using on‐chip isotachophoresis

Isolation of enriched small RNA from cell‐lysate using on‐chip isotachophoresis

<p>Long Non-Coding RNA Taurine Upregulated Gene 1 Targets miR-185 to Regulate Cell Proliferation and Glycolysis in Acute Myeloid Leukemia Cells in vitro</p>

Expression Profiling of Circulating Microvesicles Reveals Intercellular Transmission of Oncogenic Pathways

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