Your search keyword '"Primary cell lines"' showing total 34 results

1. Optimization of process parameters for specific pathogen-free chicken embryonic fibroblast cultivation for yellow fever vaccine production.

Author

Narreddy, Hareesh Reddy, Kondapalli, Ratna Prakash, and TC, Venkateswarulu

Subjects

*YELLOW fever, *CHICKENS, *FIBROBLASTS, *CELL separation, *VACCINES, *CHICKEN embryos

Abstract

AbstractThe yellow fever (YF) vaccine is usually produced with egg-based methods, which has limitations, including potential adverse effects and low production yields. Alternatively, producing the vaccine using Vero cells or HEK 293 cells can overcome some of these issues, but these methods are significantly more expensive. In the current study, the YF vaccine candidate 17DD virus was produced in primary chicken embryo fibroblast (CEF) cells. The primary CEF cells isolation from eggs was optimized through a two-step process. In the first step, the important parameters that contribute to the development of the egg embryo, such as egg position, relative humidity (RH), and incubation time are optimized. In second step, primary CEF release parameters namely; trypsin volume and incubation temperature are optimized. Both steps were optimized using statistical methods. Further, the seeding cell density of isolated CEF was also optimized. It was observed that 5 x 104 cells/cm2 gave the highest virus titer of 3.89 million PFU/ml. The 17DD yields achieved in primary CEFs are much higher than egg-based production and it is an economically viable method. [ABSTRACT FROM AUTHOR]

Published

2024

2. Characterisation of Canine and Feline Breast Tumours, Their Metastases, and Corresponding Primary Cell Lines Using LA-REIMS and DESI-MS Imaging.

Author

Molnár, Adrienn, Horkovics-Kováts, Gabriel Stefan, Kucsma, Nóra, Szegő, Zsuzsanna, Tauber, Boglárka, Egri, Attila, Szkupien, Zoltán, Deák, Bálint András, McKenzie, James S., Thuróczy, Julianna, Schäffer, Richard, Schlosser, Gitta, Szakács, Gergely, and Balog, Júlia

Subjects

*CELL lines, *TUMORS, *METASTASIS, *MASS spectrometry, *DISEASE prevalence

Abstract

Breast cancer, a complex disease with a significant prevalence to form metastases, necessitates novel therapeutic strategies to improve treatment outcomes. Here, we present the results of a comparative molecular study of primary breast tumours, their metastases, and the corresponding primary cell lines using Desorption Electrospray Ionisation (DESI) and Laser-Assisted Rapid Evaporative Ionisation Mass Spectrometry (LA-REIMS) imaging. Our results show that ambient ionisation mass spectrometry technology is suitable for rapid characterisation of samples, providing a lipid- and metabolite-rich spectrum within seconds. Our study demonstrates that the lipidomic fingerprint of the primary tumour is not significantly distinguishable from that of its metastasis, in parallel with the similarity observed between their respective primary cell lines. While significant differences were observed between tumours and the corresponding cell lines, distinct lipidomic signatures and several phospholipids such as PA(36:2), PE(36:1), and PE(P-38:4)/PE(O-38:5) for LA-REIMS imaging and PE(P-38:4)/PE(O-38:5), PS(36:1), and PI(38:4) for DESI-MSI were identified in both tumours and cells. We show that the tumours' characteristics can be found in the corresponding primary cell lines, offering a promising avenue for assessing tumour responsiveness to therapeutic interventions. A comparative analysis by DESI-MSI and LA-REIMS imaging revealed complementary information, demonstrating the utility of LA-REIMS in the molecular imaging of cancer. [ABSTRACT FROM AUTHOR]

Published

2024

3. Organoids derived from patients provide a new opportunity for research and individualized treatment of malignant peritoneal mesothelioma

Author

XiaoChang Fang, Lin Shu, TianLiang Chen, XiaoLe Zhao, LiuCui Yang, Tingting Dou, Lijie Yang, Xuanfei Li, and Maohui Feng

Subjects

Malignant peritoneal Mesothelioma, Organoids, Patient-derived organoids (PDO), Primary cell lines, Patient-derived organoids xenograft (PDOX), Peritoneal orthotopic xenograft, Neoplasms. Tumors. Oncology. Including cancer and carcinogens, RC254-282

Abstract

Abstract Background Malignant peritoneal mesothelioma (MPM) is an extremely rare and highly invasive tumor. Due to the lack of accurate models that reflect the biological characteristics of primary tumors, studying MPM remains challenging and is associated with an exceedingly unfavorable prognosis. This study was aimed to establish a new potential preclinical model for MPM using patient-derived MPM organoids (MPMOs) and to comprehensively evaluate the practicality of this model in medical research and its feasibility in guiding individualized patient treatment. Methods MPMOs were constructed using tumor tissue from MPM patients. Histopathological analysis and whole genome sequencing (WGS) were employed to determine the ability of MPMOs to replicate the original tumor's genetic and histological characteristics. The subcutaneous and orthotopic xenograft models were employed to assess the feasibility of establishing an in vivo model of MPM. MPMOs were also used to conduct drug screening and compare the results with retrospective analysis of patients after treatment, in order to evaluate the potential of MPMOs in predicting the effectiveness of drugs in MPM patients. Results We successfully established a culture method for human MPM organoids using tumor tissue from MPM patients and provided a comprehensive description of the necessary medium components for MPMOs. Pathological examination and WGS revealed that MPMOs accurately represented the histological characteristics and genomic heterogeneity of the original tumors. In terms of application, the success rate of creating subcutaneous and orthotopic xenograft models using MPMOs was 88% and 100% respectively. Drug sensitivity assays demonstrated that MPMOs have different medication responses, and these differences were compatible with the real situation of the patients. Conclusion This study presents a method for generating human MPM organoids, which can serve as a valuable research tool and contribute to the advancement of MPM research. Additionally, these organoids can be utilized as a means to evaluate the effectiveness of drug treatments for MPM patients, offering a model for personalized treatment approaches.

Published

2024

4. Organoids derived from patients provide a new opportunity for research and individualized treatment of malignant peritoneal mesothelioma

Author

Fang, XiaoChang, Shu, Lin, Chen, TianLiang, Zhao, XiaoLe, Yang, LiuCui, Dou, Tingting, Yang, Lijie, Li, Xuanfei, and Feng, Maohui

Published

2024

5. Insights into the characteristics of primary radioresistant cervical cancer using single-cell transcriptomics.

Author

Xing, Biyuan, Pu, Congli, Chen, Yunshang, Sheng, Yuhan, Zhang, Baofang, Cui, Jie, Wu, Gang, and Zhao, Yingchao

Subjects

CERVICAL cancer, CELL lines, RADIATION tolerance, CELL cycle

Abstract

Radioresistance is a major cause of radiotherapy failure among patients with cervical cancer (CC), the fourth most common cause of cancer mortality in women worldwide. Traditional CC cell lines lose intra-tumoral heterogeneity, posing a challenge for radioresistance research. Meanwhile, conditional reprogramming (CR) maintains intra-tumoral heterogeneity and complexity, as well as the genomic and clinical characteristics of original cells and tissues. Three radioresistant and two radiosensitive primary CC cell lines were developed under CR conditions from patient specimens, and their characteristics were verified via immunofluorescence, growth kinetics, clone forming assay, xenografting, and immunohistochemistry. The CR cell lines had homogenous characteristics with original tumor tissues and maintained radiosensitivity in vitro and in vivo, while also maintaining intra-tumoral heterogeneity according to single-cell RNA sequencing analysis. Upon further investigation, 20.83% of cells in radioresistant CR cell lines aggregated in the G2/M cell cycle phase, which is sensitive to radiation, compared to 38.1% of cells in radiosensitive CR cell lines. This study established three radioresistant and two radiosensitive CC cell lines through CR, which will benefit further research investigating radiosensitivity in CC. Our present study may provide an ideal model for research on development of radioresistance and potential therapeutic targets in CC. [ABSTRACT FROM AUTHOR]

Published

2023

6. TERT Extra-Telomeric Roles: Antioxidant Activity and Mitochondrial Protection.

Author

Marinaccio, Jessica, Micheli, Emanuela, Udroiu, Ion, Di Nottia, Michela, Carrozzo, Rosalba, Baranzini, Nicolò, Grimaldi, Annalisa, Leone, Stefano, Moreno, Sandra, Muzzi, Maurizio, and Sgura, Antonella

Subjects

*TELOMERES, *TELOMERASE reverse transcriptase, *MITOCHONDRIA, *CELLULAR aging, *REACTIVE oxygen species, *MEMBRANE potential, *MITOCHONDRIAL membranes

Abstract

Telomerase reverse transcriptase (TERT) is the catalytic subunit of telomerase holoenzyme, which adds telomeric DNA repeats on chromosome ends to counteract telomere shortening. In addition, there is evidence of TERT non-canonical functions, among which is an antioxidant role. In order to better investigate this role, we tested the response to X-rays and H2O2 treatment in hTERT-overexpressing human fibroblasts (HF-TERT). We observed in HF-TERT a reduced induction of reactive oxygen species and an increased expression of the proteins involved in the antioxidant defense. Therefore, we also tested a possible role of TERT inside mitochondria. We confirmed TERT mitochondrial localization, which increases after oxidative stress (OS) induced by H2O2 treatment. We next evaluated some mitochondrial markers. The basal mitochondria quantity appeared reduced in HF-TERT compared to normal fibroblasts and an additional reduction was observed after OS; nevertheless, the mitochondrial membrane potential and morphology were better conserved in HF-TERT. Our results suggest a protective function of TERT against OS, also preserving mitochondrial functionality. [ABSTRACT FROM AUTHOR]

Published

2023

7. In vivo vaccination with cell line-derived whole tumor lysates: neoantigen quality, not quantity matters

Author

Inken Salewski, Yvonne Saara Gladbach, Steffen Kuntoff, Nina Irmscher, Olga Hahn, Christian Junghanss, and Claudia Maletzki

Subjects

Tumor lysate, Mutational load, MMR deficiency, In vivo imaging, Primary cell lines, Medicine

Abstract

Abstract Background Cancer vaccines provide a complex source of neoantigens. Still, increasing evidence reveals that the neoantigen quality rather than the quantity is predictive for treatment outcome. Methods Using the preclinical Mlh1−/− tumor model, we performed a side-by side comparison of two autologous cell-line derived tumor lysates (namely 328 and A7450 T1 M1) harboring different tumor mutational burden (TMB; i.e. ultra-high: 328; moderate-high: A7450 T1 M1). Mice received repetitive prophylactic or therapeutic applications of the vaccine. Tumor incidence, immune responses and tumor microenvironment was examined. Results Both tumor cell lysates delayed tumor formation in the prophylactic setting, with the A7450 T1 M1 lysate being more effective in decelerating tumor growth than the 328 lysate (median overall survival: 37 vs. 25 weeks). Comparable results were achieved in therapeutic setting and could be traced back to antigen-driven immune stimulation. Reactive T cells isolated from A7450 T1 M1-treated mice recognized autologous Mlh1−/− tumor cells in IFNγ ELISpot, but likewise YAC-1 cells, indicative for stimulation of both arms of the immune system. By deciphering local effects, vaccines shaped the tumor microenvironment differently. While A7450 T1 M1 prophylactically vaccinated tumors harbored low numbers of myeloid-derived suppressor cells (MDSC) and elevated CD8-T cell infiltrates, vaccination with the 328 lysate evoked MDSC infiltration. Similar effects were seen in the therapeutic setting with stable disease induction only upon A7450 T1 M1 vaccination. Untangling individual response profiles revealed strong infiltration with LAG3+ and PD-L1+ immune cells when treatments failed, but almost complete exclusion of checkpoint-expressing lymphocytes in long-term survivors. Conclusions By applying two tumor cell lysates we demonstrate that neoantigen quality outranks quantity. This should be considered prior to designing cancer vaccine-based combination approaches.

Published

2020

8. The PI3K/mTOR dual inhibitor GSK458 potently impedes ovarian cancer tumorigenesis and metastasis.

Author

Xiao, Yangjiong, Yu, Yang, Jiang, Pengcheng, Li, Yuhong, Wang, Chao, and Zhang, Rong

Subjects

*OVARIAN cancer, *METASTASIS, *CANCER cell migration, *GRAFTING (Horticulture), *MTOR inhibitors, *CELL cycle

Abstract

Purpose: The PI3K/AKT/mTOR pathway is one of the most highly activated cellular signaling pathways in advanced ovarian cancer. Although several PI3K/AKT/mTOR inhibitors have been developed to treat various types of cancer, the antitumor efficacy of many of these compounds against ovarian cancer has remained unclear. Methods: Here, we tested and compared a panel of 16 PI3K/AKT/mTOR inhibitors (XL765, Miltefosine, Rapamycin, CCI-779, RAD001, FK506, XL147, GSK2110183, IPI-145, GSK2141795, BYL719, GSK458, CAL-101, XL765 analogue SAR245409, Triciribine, and GDC0941) that have entered clinical trials for antitumor activity against ovarian cancer, as well as the front line drug, paclitaxel. Antitumor efficacy was measured in both ovarian cancer cell lines and patient-derived ovarian primary tumor cell lines in vitro and in vivo. Results: We identified the PI3K/mTOR dual inhibitor GSK458 as a potent inhibitor of proliferation in all cell lines tested at half maximal inhibitory concentrations (IC50) of approximately 0.01-1 µM, a range tens to hundreds fold lower than that of the other PI3K/AKT/mTOR inhibitors tested. Additionally, GSK458 showed the highest inhibitory efficacy against ovarian cancer cell migration. GSK458 also inhibited tumor growth and metastasis in nude mice intraperitoneally engrafted with SKOV3 cells or a patient-derived tumor cell xenograft (PDCX). Importantly, the inhibitory efficiency of GSK458 on cell proliferation and migration both in vitro and in vivo was comparable to that of paclitaxel. Mechanistically, the anti-tumor activity of GSK458 was found to be associated with inactivation of AKT and mTOR, and induction of cell cycle arrest at the G0/G1 phase. Conclusions: Based on our results, we conclude that GSK458 may serve as an attractive candidate to treat ovarian cancer. [ABSTRACT FROM AUTHOR]

Published

2020

9. Inhibition of CDC25B With WG-391D Impedes the Tumorigenesis of Ovarian Cancer

Author

Yangjiong Xiao, Yang Yu, Dan Gao, Wangrui Jin, Pengcheng Jiang, Yuhong Li, Chao Wang, Yuning Song, Peng Zhan, Fei Gu, Cancan Zhang, Bin Wang, Yihua Chen, Bing Du, and Rong Zhang

Subjects

WG-391D, ovarian cancer, PDX, primary cell lines, target therapy, Neoplasms. Tumors. Oncology. Including cancer and carcinogens, RC254-282

Abstract

Novel inhibitors are urgently needed for use as targeted therapies to improve the overall survival (OS) of patients with ovarian cancer. Here, we show that cell division cycle 25B (CDC25B) is over-expressed in ovarian tumors and associated with poor patient prognosis. All previously reported CDC25B inhibitors have been identified by their ability to reversibly inhibit the catalytic dephosphorylation activity of CDC25B in vitro; however, none of these compounds have entered clinical trials for ovarian cancer therapy. In this study, we synthesized a novel small molecule compound, WG-391D, that potently down-regulates CDC25B expression without affecting its catalytic dephosphorylation activity. The inhibition of CDC25B by WG-391D is irreversible, and WG-391D should therefore exhibit potent antitumor activity against ovarian cancer. WG-391D induces cell cycle progression arrest at the G2/M phase. Half maximal inhibitory concentration (IC50) values of WG-391D for inhibition of the proliferation and migration of eight representative ovarian cancer cell lines (SKOV3, ES2, OVCAR8, OVTOKO, A2780, IGROV1, HO8910PM, and MCAS) and five primary ovarian tumor cell lines (GFY004, GFY005, CZ001, CZ006, and CZ008) were lower than 10 and 1 μM, respectively. WG-391D inhibited tumor growth in nude mice inoculated with SKOV3 cells or a patient-derived xenograft (PDX). The underlying mechanisms were associated with the down-regulation of CDC25B and subsequent inactivation of cell division cycle 2 (CDC2) and the serine/threonine kinase, AKT. In conclusion, this study demonstrates that WG-391D exhibits strong antitumor activity against ovarian cancer and indicates that the down-regulation of CDC25B by inhibitors could provide a rationale for ovarian cancer therapy.

Published

2019

10. Canine oral primary melanoma cells exhibit shift to mesenchymal phenotype and phagocytic behaviour.

Author

Schmid, Franziska, Brodesser, Daniela, Reifinger, Martin, Forte, Sara, Semp, Pia, Eberspächer‐Schweda, Matthias C., Wolschek, Markus, Brandt, Sabine, Kleiter, Miriam, and Pratscher, Barbara

Subjects

*PRIMARY cell culture, *MELANOMA, *CELL lines, *PHAGOCYTIC function tests, *BEHAVIOR, *PHAGOCYTOSIS

Abstract

Canine oral malignant melanoma (COMM) is a potentially lethal cancer disease. We established primary cell lines from mostly amelanotic primary COMM and metastases and assessed lesions and derived cells for Melan A, PNL2 and CD146 expression. Then, migration and invasion of CD146‐enriched vs ‐depleted COMM cells were analysed. Epithelial‐to‐mesenchymal transition (EMT) was addressed by Vimentin‐staining and MMP2/MMP9 zymography. Phagocytic behaviour was analysed by histopathological examination and phagocytosis assay. While Melan A‐ and PNL2‐staining yielded inconsistent data, 100% of COMM sections and primary cells showed CD146 expression, suggesting that this protein may serve as a prognostic marker. An overall correlation between CD146‐expression and migration/invasion was not observed. All primary cell lines consistently expressed Vimentin and secreted biologically active MMP2, indicating that they had undergone EMT. Importantly, COMM sections exhibited cell‐in‐cell structures, and all primary cell lines exhibited phagocytic activity, supporting the concept that cell cannibalism may have a role in COMM progression. [ABSTRACT FROM AUTHOR]

Published

2019

11. Inhibition of CDC25B With WG-391D Impedes the Tumorigenesis of Ovarian Cancer.

Author

Xiao, Yangjiong, Yu, Yang, Gao, Dan, Jin, Wangrui, Jiang, Pengcheng, Li, Yuhong, Wang, Chao, Song, Yuning, Zhan, Peng, Gu, Fei, Zhang, Cancan, Wang, Bin, Chen, Yihua, Du, Bing, and Zhang, Rong

Subjects

OVARIAN cancer treatment, NEOPLASTIC cell transformation, CELL division, ANTINEOPLASTIC agents, DEPHOSPHORYLATION

Abstract

Novel inhibitors are urgently needed for use as targeted therapies to improve the overall survival (OS) of patients with ovarian cancer. Here, we show that cell division cycle 25B (CDC25B) is over-expressed in ovarian tumors and associated with poor patient prognosis. All previously reported CDC25B inhibitors have been identified by their ability to reversibly inhibit the catalytic dephosphorylation activity of CDC25B in vitro ; however, none of these compounds have entered clinical trials for ovarian cancer therapy. In this study, we synthesized a novel small molecule compound, WG-391D, that potently down-regulates CDC25B expression without affecting its catalytic dephosphorylation activity. The inhibition of CDC25B by WG-391D is irreversible, and WG-391D should therefore exhibit potent antitumor activity against ovarian cancer. WG-391D induces cell cycle progression arrest at the G2/M phase. Half maximal inhibitory concentration (IC50) values of WG-391D for inhibition of the proliferation and migration of eight representative ovarian cancer cell lines (SKOV3, ES2, OVCAR8, OVTOKO, A2780, IGROV1, HO8910PM, and MCAS) and five primary ovarian tumor cell lines (GFY004, GFY005, CZ001, CZ006, and CZ008) were lower than 10 and 1 μM, respectively. WG-391D inhibited tumor growth in nude mice inoculated with SKOV3 cells or a patient-derived xenograft (PDX). The underlying mechanisms were associated with the down-regulation of CDC25B and subsequent inactivation of cell division cycle 2 (CDC2) and the serine/threonine kinase, AKT. In conclusion, this study demonstrates that WG-391D exhibits strong antitumor activity against ovarian cancer and indicates that the down-regulation of CDC25B by inhibitors could provide a rationale for ovarian cancer therapy. [ABSTRACT FROM AUTHOR]

Published

2019

12. Oxaliplatin and irinotecan induce heterogenous changes in the EMT markers of metastasizing colorectal carcinoma cells.

Author

Skarkova, Veronika, Kralova, Vera, Krbal, Lukas, Matouskova, Petra, Soukup, Jiri, and Rudolf, Emil

Subjects

*OXALIPLATIN, *COLON cancer treatment, *CANCER chemotherapy, *CELL-mediated cytotoxicity, *WESTERN immunoblotting, *THERAPEUTICS

Abstract

In patients with advanced colorectal cancer (CRC), surgery is complemented with systemic therapy – chemotherapy and radiochemotherapy. Although the patients’ overall survival has been significantly improved, tumor resistance is still a frequent cause of chemotherapy failure. Several factors contribute to chemoresistance of tumor cells including changes related with epithelial-mesenchymal transition (EMT). The present study was designed to verify the presence of EMT markers in paired CRC primary cell lines obtained from primary tumor sites and lymph node metastases of three patients and to investigate the effect of irinotecan and oxaliplatin treatment on these markers as well. The samples of the higher stage of CRC and positive for angioinvasion were selected and qPCR, western blot analysis, migration assay, cytotoxicity testing was performed. Results confirmed the increased expression of several markers characteristic of EMT and invasiveness in lymph node metastatic cells, with a significant variability between individual samples. Irinotecan and oxaliplatin decreased migration activity of the cells and to the varying degree affected the expression of EMT and invasiveness markers. In conclusion, in CRC EMT is present in metastatic cells over a phenotypic continuum whose expression is altered heterogeneously upon irinotecan and oxaliplatin treatment. [ABSTRACT FROM AUTHOR]

Published

2018

13. "Simple Methods to Derive Primary Malignant Glioma Cell Lines and Assay of Cellular Damage for Preclinical Studies".

Author

Thakur, Kalyani, Shyam, Sai, George, Jennifer, A. G., Shobha, Rao, K. V. L. Narasinga, and Kalia, Vijay Kumar

Subjects

*GLIOMAS, *CELL lines, *ANTINEOPLASTIC agents, *CHEMORADIOTHERAPY, *CELL death, *APOPTOSIS, *BIOLOGICAL assay, *BRAIN tumors, *CELL culture, *CELL physiology, *DRUG design, *CLINICAL drug trials, *GAMMA rays, *RADIATION doses, *CANCER cell culture, *TUMOR grading, *PHARMACODYNAMICS, *PHYSIOLOGICAL effects of radiation

Abstract

Primary malignant glioma cell lines are being used for initial screening of anticancer agents. We utilized a simple mechanical disaggregation method for deriving cell lines from tumor tissues; and a Coverslip Culture-Acridine Orange Staining method to study cellular damage. Cell lines could be grown for up to three passages within three weeks after surgery. Cell proliferation, total cellular damage, and MTT assay were studied as parameters of cytotoxic response. Frequencies of damaged cells varied in different cell lines; and increased after cytotoxic treatments under clinically relevant conditions. These methods could contribute to preclinical evaluation of treatment response before commencement of radio-chemotherapy. [ABSTRACT FROM AUTHOR]

Published

2018

14. Biomarkers of prostate cancer sensitivity to the Sendai virus.

Author

Belova, A., Sosnovtseva, A., Lipatova, A., Njushko, K., Volchenko, N., Belyakov, M., Sudalenko, O., Krasheninnikov, A., Shegai, P., Sadritdinova, A., Fedorova, M., Vorobjov, N., Alekseev, B., Kaprin, A., and Kudryavtseva, A.

Subjects

*PROSTATE cancer, *SENDAI virus, *GENE expression, *ADENOCARCINOMA

Abstract

Metastatic prostate cancer is often associated with either primary or intractable castration-resistant prostate cancer (CRPC), thus justifying the search for entirely new ways of treatment. Oncolytic viruses are able to selectively induce the death of tumor cells without affecting normal cells. A murine Sendai virus has potential to be used as an oncolytic agent. However, tumors vary in their sensitivity to different viruses, prompting us to attempt to identify corresponding biomarkers that reflect the interaction of cancer cells and the virus. Here, we show that the sensitivity of primary prostatic adenocarcinoma cell lines to Sendai virus strain (SeVM) vary substantially. Using quantitative PCR, we evaluated expression levels of genes that encode RIG-1-like and Toll-like receptors (TLRs) in cell lines and showed that the levels of mRNAs that encode TLR3 and TLR7 correlate with a degree of sensitivity of the cells to Sendai virus. The lines with lower levels of TLR3 and TLR7 expression are more sensitive to the virus. [ABSTRACT FROM AUTHOR]

Published

2017

15. TERT Extra-Telomeric Roles: Antioxidant Activity and Mitochondrial Protection

Author

Jessica Marinaccio, Emanuela Micheli, Ion Udroiu, Michela Di Nottia, Rosalba Carrozzo, Nicolò Baranzini, Annalisa Grimaldi, Stefano Leone, Sandra Moreno, Maurizio Muzzi, Antonella Sgura, Marinaccio, Jessica, Micheli, Emanuela, Udroiu, Ion, Di Nottia, Michela, Carrozzo, Rosalba, Baranzini, Nicolò, Grimaldi, Annalisa, Leone, Stefano, Moreno, Sandra, Muzzi, Maurizio, and Sgura, Antonella

Subjects

electron microscopy, Organic Chemistry, General Medicine, telomerase catalytic subunit, Catalysis, primary cell lines, Computer Science Applications, Inorganic Chemistry, primary cell line, mitochondrion, oxidative response, Physical and Theoretical Chemistry, Molecular Biology, Spectroscopy

Abstract

Telomerase reverse transcriptase (TERT) is the catalytic subunit of telomerase holoenzyme, which adds telomeric DNA repeats on chromosome ends to counteract telomere shortening. In addition, there is evidence of TERT non-canonical functions, among which is an antioxidant role. In order to better investigate this role, we tested the response to X-rays and H2O2 treatment in hTERT-overexpressing human fibroblasts (HF-TERT). We observed in HF-TERT a reduced induction of reactive oxygen species and an increased expression of the proteins involved in the antioxidant defense. Therefore, we also tested a possible role of TERT inside mitochondria. We confirmed TERT mitochondrial localization, which increases after oxidative stress (OS) induced by H2O2 treatment. We next evaluated some mitochondrial markers. The basal mitochondria quantity appeared reduced in HF-TERT compared to normal fibroblasts and an additional reduction was observed after OS; nevertheless, the mitochondrial membrane potential and morphology were better conserved in HF-TERT. Our results suggest a protective function of TERT against OS, also preserving mitochondrial functionality.

Published

2023

16. Selective isolation and characterization of primary cells from normal breast and tumors reveal plasticity of adipose derived stem cells.

Author

Weigand, Annika, Boos, Anja M., Tasbihi, Kereshmeh, Beier, Justus P., Dalton, Paul D., Schrauder, Michael, Horch, Raymund E., Beckmann, Matthias W., Strissel, Pamela L., and Strick, Reiner

Subjects

CELL lines, BREAST tumors, BREAST cancer, STEM cells, GENE expression, BREAST, CELL culture, CELL physiology, CONNECTIVE tissue cells, CULTURE media (Biology), EPITHELIAL cells, FAT cells, PROTEINS

Abstract

Background: There is a need to establish more cell lines from breast tumors in contrast to immortalized cell lines from metastatic effusions in order to represent the primary tumor and not principally metastatic biology of breast cancer. This investigation describes the simultaneous isolation, characterization, growth and function of primary mammary epithelial cells (MEC), mesenchymal cells (MES) and adipose derived stem cells (ADSC) from four normal breasts, one inflammatory and one triple-negative ductal breast tumors.Methods: A total of 17 cell lines were established and gene expression was analyzed for MEC and MES (n = 42) and ADSC (n = 48) and MUC1, pan-KRT, CD90 and GATA-3 by immunofluorescence. DNA fingerprinting to track cell line identity was performed between original primary tissues and isolates. Functional studies included ADSC differentiation, tumor MES and MEC invasion co-cultured with ADSC-conditioned media (CM) and MES adhesion and growth on 3D-printed scaffolds.Results: Comparative analysis showed higher gene expression of EPCAM, CD49f, CDH1 and KRTs for normal MEC lines; MES lines e.g. Vimentin, CD10, ACTA2 and MMP9; and ADSC lines e.g. CD105, CD90, CDH2 and CDH11. Compared to the mean of all four normal breast cell lines, both breast tumor cell lines demonstrated significantly lower ADSC marker gene expression, but higher expression of mesenchymal and invasion gene markers like SNAI1 and MMP2. When compared with four normal ADSC differentiated lineages, both tumor ADSC showed impaired osteogenic and chondrogenic but enhanced adipogenic differentiation and endothelial-like structures, possibly due to high PDGFRB and CD34. Addressing a functional role for overproduction of adipocytes, we initiated 3D-invasion studies including different cell types from the same patient. CM from ADSC differentiating into adipocytes induced tumor MEC 3D-invasion via EMT and amoeboid phenotypes. Normal MES breast cells adhered and proliferated on 3D-printed scaffolds containing 20 fibers, but not on 2.5D-printed scaffolds with single fiber layers, important for tissue engineering.Conclusion: Expression analyses confirmed successful simultaneous cell isolations of three different phenotypes from normal and tumor primary breast tissues. Our cell culture studies support that breast-tumor environment differentially regulates tumor ADSC plasticity as well as cell invasion and demonstrates applications for regenerative medicine. [ABSTRACT FROM AUTHOR]

Published

2016

17. In vivo vaccination with cell line-derived whole tumor lysates: neoantigen quality, not quantity matters

Author

Salewski, Inken, Gladbach, Yvonne Saara, Kuntoff, Steffen, Irmscher, Nina, Hahn, Olga, Junghanss, Christian, and Maletzki, Claudia

Published

2020

18. Cytotoxic and Genotoxic Effects of Arsenic on Primary Human Breast Cancer Cell Lines.

Author

Ahmad, Aftab, Ashraf, Sadia, and Shakoori, A. R.

Abstract

Breast cancer is one of the most common cancers, with high incidence rate among women Prevalence of breast cancer in Pakistan is highest in Asia. The present study was done to observe the effect of arsenic on breast cancer cell lines that was locally established Breast cancer tissues were taken from two hospitals and primary breast cancer cell lines were established by explants culture method. Neutral red based anti-proliferative assays were done to check the effect of arsenic on Pakistan Breast Cancer INMOL (PBCI) and Pakistan Breast Cancer Jinnali (PBCJ) cell lines. Comet assay was done to check the genotoxic effect of arsenic. Letal concentration 50 (LC50) for PBCI was 13 µ/ml on 24 h exposure and it shifted to 12 µ/ml when the cells were exposed for 48 h, while LC50, for PBCJ was 9 µ/ml. PBCJ cells proved to be more sensitive to arsenic than PBCI. When the number of cells were increased (1x104 cells per well) in 96 well plate LC50 for PBCI was 19 µ/ml. There was comet formation in arsenic treated samples compared to control. Ten different parameters were investigated for arsenic treated and control cells. The results indicated that arsenic had great cytotoxic and genotoxic effect on breast cancer cells and morphology of cells was totally changed with higher concentrations (12 µ/ml or higher) of arsenic. [ABSTRACT FROM AUTHOR]

Published

2015

19. Achimota Pararubulavirus 3: A New Bat-Derived Paramyxovirus of the Genus Pararubulavirus

Author

Gary Crameri, Mary Tachedjian, Ina Smith, Andrés Fernández-Loras, Shawn Todd, James L. N. Wood, Andrew A. Cunningham, Glenn A. Marsh, Richard Suu-Ire, Jennifer A. Barr, Sandra Crameri, Lin-Fa Wang, Clare Holmes, Kate S. Baker, Wood, James [0000-0002-0258-3188], and Apollo - University of Cambridge Repository

Subjects

0301 basic medicine, Old World, animal structures, Paramyxoviridae, 030106 microbiology, lcsh:QR1-502, Genomics, bat, Genome, Viral, virus, Kidney, Genome, lcsh:Microbiology, primary cell lines, 03 medical and health sciences, paramyxovirus, Genus, Chiroptera, Zoonoses, Virology, Chlorocebus aethiops, medicine, genomics, Animals, Vero Cells, Cells, Cultured, Phylogeny, virus discovery, Paramyxoviridae Infections, Whole Genome Sequencing, Phylogenetic tree, biology, electron microscopy, Transmission (medicine), Zoonosis, zoonosis, biology.organism_classification, medicine.disease, molecular detection, 030104 developmental biology, Infectious Diseases, Evolutionary biology, pararubulavirus, Paramyxovirinae, RNA, Viral

Abstract

Bats are an important source of viral zoonoses, including paramyxoviruses. The paramyxoviral Pararubulavirus genus contains viruses mostly derived from bats that are common, diverse, distributed throughout the Old World, and known to be zoonotic. Here, we describe a new member of the genus Achimota pararubulavirus 3 (AchPV3) and its isolation from the urine of African straw-coloured fruit bats on primary bat kidneys cells. We sequenced and analysed the genome of AchPV3 relative to other Paramyxoviridae, revealing it to be similar to known pararubulaviruses. Phylogenetic analysis of AchPV3 revealed the failure of molecular detection in the urine sample from which AchPV3 was derived and an attachment protein most closely related with AchPV2&mdash, a pararubulavirus known to cause cross-species transmission. Together these findings add to the picture of pararubulaviruses, their sources, and variable zoonotic potential, which is key to our understanding of host restriction and spillover of bat-derived paramyxoviruses. AchPV3 represents a novel candidate zoonosis and an important tool for further study.

Published

2020

20. Achimota Pararubulavirus 3: A New Bat-Derived Paramyxovirus of the Genus

Author

Kate S, Baker, Mary, Tachedjian, Jennifer, Barr, Glenn A, Marsh, Shawn, Todd, Gary, Crameri, Sandra, Crameri, Ina, Smith, Clare E G, Holmes, Richard, Suu-Ire, Andres, Fernandez-Loras, Andrew A, Cunningham, James L N, Wood, and Lin-Fa, Wang

Subjects

virus discovery, animal structures, Paramyxoviridae Infections, Whole Genome Sequencing, electron microscopy, bat, Genome, Viral, virus, zoonosis, Kidney, Article, primary cell lines, molecular detection, paramyxovirus, Chiroptera, Zoonoses, pararubulavirus, Chlorocebus aethiops, genomics, Animals, Paramyxovirinae, RNA, Viral, Vero Cells, Cells, Cultured, Phylogeny

Abstract

Bats are an important source of viral zoonoses, including paramyxoviruses. The paramyxoviral Pararubulavirus genus contains viruses mostly derived from bats that are common, diverse, distributed throughout the Old World, and known to be zoonotic. Here, we describe a new member of the genus Achimota pararubulavirus 3 (AchPV3) and its isolation from the urine of African straw-coloured fruit bats on primary bat kidneys cells. We sequenced and analysed the genome of AchPV3 relative to other Paramyxoviridae, revealing it to be similar to known pararubulaviruses. Phylogenetic analysis of AchPV3 revealed the failure of molecular detection in the urine sample from which AchPV3 was derived and an attachment protein most closely related with AchPV2—a pararubulavirus known to cause cross-species transmission. Together these findings add to the picture of pararubulaviruses, their sources, and variable zoonotic potential, which is key to our understanding of host restriction and spillover of bat-derived paramyxoviruses. AchPV3 represents a novel candidate zoonosis and an important tool for further study.

Published

2020

21. Establishment and Histopathological Study of Patient-derived Xenograft Models and Primary Cell Lines of Epithelioid Malignant Peritoneal Mesothelioma

Author

Ru Ma, Zhong-He Ji, Zhi-Gao Chen, Zhao Li, Zhi-Ran Yang, Xi Jiang, Jue Zhang, Yulin Lin, Yan Li, Qian Chen, and Xue-Mei Du

Subjects

Male, Pathology, medicine.medical_specialty, Original, H&E stain, Mice, Nude, histopathological study, Immunofluorescence, Peritoneal Diseases, General Biochemistry, Genetics and Molecular Biology, primary cell lines, whole exome sequencing, Gross examination, Cytokeratin, Mice, Cell Line, Tumor, Medicine, Animals, Humans, patient-derived xenograft (PDX) model, Mesothelioma, BAP1, General Veterinary, medicine.diagnostic_test, business.industry, Epithelioid Cells, Mesothelioma, Malignant, General Medicine, Middle Aged, medicine.disease, Disease Models, Animal, malignant peritoneal mesothelioma, Peritoneal Cancer Index, Immunohistochemistry, Heterografts, Animal Science and Zoology, Female, business

Abstract

Background: Malignant peritoneal mesothelioma (MPM) is a rare malignancy with few effective therapies. This study established patient-derived xenograft (PDX) models and primary cell lines to provide a study platform for MPM in vitro and in vivo, and conducted histopathological analysis.Methods: Human MPM surgical specimen was collected to establish PDX models and primary cell lines. Experimental peritoneal cancer index (ePCI) score was used to evaluate gross pathology, and histopathological study was conducted by hematoxylin-eosin (HE) and immunohistochemistry (IHC) staining. Pathological characteristics of the established primary MPM cell lines were analyzed by Swiss-Gimsa and immunofluorescence (IF) staining. The whole-exome sequencing (WES) was performed to identify the mutant genes between models and the patient.Results: MPM PDX models and primary cell lines were successfully established, replicated the pathological features of the patient. ePCI score of the female and male nude mice were 8.80 ± 1.75 and 9.20 ± 1.81 (P = 0.6219), respectively. The HE staining showed that the tumor was epithelioid mesothelioma and invaded multiple organs. IHC staining showed that Calretinin, Cytokeratin 5/6, WT-1 and Ki-67 were all positive. The Swiss-Gimsa and IF staining of primary cell lines were also consistent with the pathological characteristics of mesothelioma. The WES showed that 21 mutant genes were shared between models and the patient, and the genes related to tumorigenesis and development including BAP1, NF2, MTBP, NECTIN2, CDC23, LRPPRC, TRIM25, and DHRS2.Conclusions: PDX models and primary cell lines of MPM were successfully established with the epithelioid mesothelioma identity confirmed by histopathological evidence. Moreover, our study has also illustrated the shared genomic profile between models and the patient, then potentially provided new targets for MPM treatment.

Published

2020

22. PD-L1 assessment in pediatric rhabdomyosarcoma: a pilot study

Author

Patrizia Gasparini, Michela Casanova, Salvatore Lorenzo Renne, Stefano Chiaravalli, Luca Bergamaschi, Andrea Ferrari, Marta Barisella, Paola Collini, Massimo Milione, Cinzia Paolino, Cecilia Gardelli, Maura Massimino, Giulia Bertolini, and Giovanni Centonze

Subjects

Male, 0301 basic medicine, Cancer Research, Pathology, medicine.medical_specialty, Pilot Projects, Soft Tissue Neoplasms, PD-L1 expression, lcsh:RC254-282, B7-H1 Antigen, Flow cytometry, 03 medical and health sciences, 0302 clinical medicine, Immune system, PD-L1, Rhabdomyosarcoma, Biomarkers, Tumor, Genetics, Humans, Medicine, Child, Retrospective Studies, Soft tissue sarcoma, Primary cell lines, biology, medicine.diagnostic_test, business.industry, Immunohistrochemistry, medicine.disease, lcsh:Neoplasms. Tumors. Oncology. Including cancer and carcinogens, Immune checkpoint, Pediatric malignancies, 030104 developmental biology, Oncology, 030220 oncology & carcinogenesis, biology.protein, Immunohistochemistry, Female, Antibody, business, Research Article

Abstract

Background Rhabdomyosarcomas (RMSs) are the most frequent soft tissue sarcoma in children and adolescents, defined by skeletal muscle differentiation and the status of FOXO1 fusions. In pediatric malignancies, in particular RMS, scant and controversial observations are reported about PD-L1 expression as a putative biomarker and few immune checkpoint clinical trials are conducted. Methods PD-L1 assessment was evaluated by immunohistochemistry (IHC) utilizing two anti-PDL1 antibodies, in a pilot cohort of 25 RMS. Results were confirmed in primary and commercial RMS cell lines by cytofluorimetric analysis and IHC. Results PD-L1 expression was detectable, by both anti-PD-L1 antibodies, in the immune contexture of immune cells infiltrating and/or surrounding the tumor, in 15/25 (60%) RMS, while absent expression was observed in neoplastic cells. Flow cytometry analysis and PD-L1 IHC of commercial and primary RMS cell lines confirmed a very small percentage of PD-L1 positive-tumor cells, under the detection limits of conventional IHC. Interestingly, increased PD-L1 expression was observed in the immune contexture of 4 RMS cases post chemotherapy compared to their matched pre-treatment samples. Conclusion Here we identify a peculiar pattern of PD-L1 expression in our RMS series with scanty positive-tumor cells detected by flow cytometry, and recurrent expression in the immune cells surrounding or infiltrating the tumor burden. Electronic supplementary material The online version of this article (10.1186/s12885-018-4554-8) contains supplementary material, which is available to authorized users.

Published

2018

23. Biological heterogeneity of primary cancer-associated fibroblasts determines the breast cancer microenvironment.

Author

Musielak M, Piwocka O, Kulcenty K, Ampuła K, Adamczyk B, Piotrowski I, Fundowicz M, Kruszyna-Mochalska M, Suchorska WM, and Malicki J

Abstract

Cancer-associated fibroblasts are a highly heterogeneous group of cells whose phenotypes and gene alterations are still under deep investigation. As a part of tumor microenvironment, they are the focus of a growing number of studies. Cancer-associated fibroblasts might become a new target of breast cancer therapy, but still more tests and analyses are needed to understand mechanisms and interactions between them and breast cancer cells. The study aimed to isolate cancer associated fibroblasts from breast cancer tissue and to phenotype the isolated cell lines. We focused on various cancer-associated fibroblast characteristic biomarkers and those that might differentiate various cancer-associated fibroblasts' subtypes. Patients with a histological diagnosis of invasive breast cancer (diameter ≤15 mm) and qualified for primary surgical treatment were enrolled in the study. Cell lines were isolated from breast cancer biopsy. For the phenotyping, we used flow cytometry, immunofluorescence and RT-qPCR analysis. Based on our study, there was no indication of a clear pattern in the cancer-associated fibroblasts' classification. Results of cancer-associated fibroblasts expression were highly heterogeneous, and specific subtypes were not defined. Moreover, comparing cancer-associated fibroblasts divided into groups based on BC subtypes from which they were isolated also did not allow to notice of any clear pattern of expressions. In the future, a higher number of analyzed cancer-associated fibroblast cell lines should be investigated to find expression schemes., Competing Interests: The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest., (AJCR Copyright © 2022.)

Published

2022

24. Isolation and Culture of Vascular Distal Outflow Pathway (VDOP) Cells From Human Donor Eyes.

Author

Roy Chowdhury U and Fautsch MP

Subjects

Aqueous Humor metabolism, Humans, Sclera metabolism, Trabecular Meshwork metabolism, Glaucoma metabolism, Intraocular Pressure

Abstract

Glaucoma, a progressive neurodegenerative ocular disease, is the leading cause of irreversible blindness worldwide. Elevated intraocular pressure (IOP) is the most common-and the only treatable-risk factor for glaucoma. IOP is generated by the balance between production and removal of aqueous humor in the anterior part of the eye, and the latter happens either through the uveoscleral or the conventional pathway. Although both pathways are important for aqueous humor removal, dysfunction within the conventional pathway is more commonly associated with increased resistance leading to elevated IOP and glaucoma. The conventional pathway can be separated into proximal (trabecular meshwork and inner wall of Schlemm's canal) and distal (outer wall of Schlemm's canal, collector channels, and episcleral vasculature) regions. Both regions contribute resistance to aqueous humor removal, but the proximal region has been studied more extensively due to the availability of model systems. In contrast, little is known about the role of the distal region in outflow resistance, largely due to the lack of suitable in vitro models. To address this, we have developed a novel method of isolating and culturing vascular distal outflow pathway (VDOP) cells from the distal outflow region of human eyes. VDOP cells can be used to study the physiological and molecular functions of cells in the distal outflow region and can help in the development of ocular hypotensive drugs that specifically target this area. We also provide a protocol describing immunohistochemical methods to validate the molecular profile of these cells, utilizing cell surface markers that distinguish them from adjacent cells. © 2022 Wiley Periodicals LLC. Basic Protocol 1: Isolation and culture of VDOP cells Basic Protocol 2: Analysis of cell surface markers., (© 2022 Wiley Periodicals LLC.)

Published

2022

25. Efficient polycation non-viral gene delivery system with high buffering capacity and low molecular weight for primary cells: Branched poly(β-aminoester) containing primary, secondary and tertiary amine groups.

Author

Gök, Mehmet Koray, Demir, Kamber, Cevher, Erdal, Pabuccuoğlu, Serhat, and Özgümüş, Saadet

Subjects

*TERTIARY amines, *MOLECULAR weights, *SECONDARY amines, *MICHAEL reaction, *POLYCONDENSATION, *GENETIC transformation

Abstract

[Display omitted] • Transfection efficiency of PBAE on primary cells was realized for the first time. • Nanoparticles prepared with DMSO have more stable than those prepared with ethanol. • More pEGFN1 were loaded into the nanoparticle with the encapsulation method. • Nanoparticles loaded pEGFN1 by encapsulation increased the transfection efficiency. • The presence of three amine structures on PBAE increased transfection efficiency. Gene transfer studies, preferred in many biotechnology studies such as in vitro transgenic cell modeling systems, gene therapy, transgenic animal production by cloning, etc., are quite limited due to transfection difficulties on primary cell lines. The main purpose of this study is on the production of biocompatible gene carrier systems with high transfection efficiency for Primary Ovine Fibroblast cell lines (POF). To achieve this goal, the synthesis of the branched poly(β-aminoester) (PBAE) containing primary, secondary and tertiary amino groups in their molecular structures was carried out via step-growth polymerization by a typical Michael addition reaction between bisphenol A-ethoxylate diacrylate (BPAEDA) and ethylenediamine (EDA) for the first time. PBAEs were characterized using FTIR and NMR techniques. GPC-SEC system was used to determine the molecular weight of these polymers. Proton buffering capacity of the PBAE was also determined. In order to optimize the preparation of the PBAE nanoparticles (nPBAE), two different methods, which are solvent evaporation and solvent displacement techniques, were used. Their physicochemical properties such as particle size, polydispersity index (PDI), zeta potential and stability were identified. nPBAE-gene complexes (gnPBAE) were obtained according to the adsorption or encapsulation mechanisms and their properties were evaluated by comparative surface charge and gel electrophoresis. In vitro studies including gene binding capacity, cytotoxicity and the transfection efficiency for primary ovine fibroblast (POF) cell lines were also realized. Consequently, (egnPBAE) dw formulation, which is obtained from PBAE EDA with the lowest Mw by encapsulation method in this study, have very high in vitro transfection efficiency up to 78.3% in POF cells and it was also exhibited almost 1.5 times more transfection efficiency against commercial product Lipofectamine because of its low M w and the presence of the secondary and tertiary amine structures as well as primary amine end groups in its backbone. [ABSTRACT FROM AUTHOR]

Published

2022

26. A method for prolonged survival of primary cell lines.

Author

Horisberger, Michel

Abstract

We have established a means for prolonged survival of primary cell cultures and establishment of continuous cell lines without genetic manipulations. Primary cultures of granulosa cells degenerate rapidly in vitro by a spontaneous onset of apoptotic cell death. Earlier attempts to circumvent this limitation have included transformation with oncogenes, spontaneous immortalization of primary cultures, and chemical carcinogenesis. We have found that addition of a complex of growth-promoting compounds, carrier proteins, and factors isolated from porcine follicular fluid to standard culture medium allows, reproducibly, the establishment of continuous porcine primary granulosa cell lines with genetic stability. This same supplement allows the prolonged survival of primary cell cultures derived from adult rat ovaries. The rat ovary primary cultures consisted of mixed phenotypes, including epithelial, neuron-like, and mesenchymal cell types. Numerous cells stain positive for alkaline phosphatase in these cultures. Other primary cell lines were established from embryonic rat liver and from adult rat lungs, using the same supplement. The survival effect is reversible because cells degenerate when the supplement is removed. Therefore, the cell lines have neither acquired properties of a tumor cell line nor have they been immortalized by a virus infection. We expect that our approach will open the door to prolonged survival of other primary cell types. [ABSTRACT FROM AUTHOR]

Published

2006

27. PD-L1 assessment in pediatric rhabdomyosarcoma: a pilot study

Author

Bertolini, Giulia, Bergamaschi, Luca, Ferrari, Andrea, Renne, Salvatore L., Collini, Paola, Gardelli, Cecilia, Barisella, Marta, Centonze, Giovanni, Chiaravalli, Stefano, Paolino, Cinzia, Milione, Massimo, Massimino, Maura, Casanova, Michela, and Gasparini, Patrizia

Published

2018

28. New Chondrosarcoma Cell Lines with Preserved Stem Cell Properties to Study the Genomic Drift During In Vitro/In Vivo Growth

Author

Laura Santos, Aida Rodríguez, Aurora Astudillo, Carlos Alvarez-Fernandez, Rene Rodriguez, Oscar Estupiñan, Juan Tornín, David Castillo, Serafín Costilla, Sofía T. Menéndez, Lucia Martinez-Cruzado, Alejandro Braña, Gonzalo R. Ordóñez, and Veronica Rey

Subjects

cancer stem cells, IDH1, lcsh:Medicine, IDH2, Article, primary cell lines, whole exome sequencing, 03 medical and health sciences, 0302 clinical medicine, Cancer stem cell, CDKN2A, medicine, 030304 developmental biology, chondrosarcoma, 0303 health sciences, business.industry, animal model, lcsh:R, genomic drift, cancer preclinical model, Cancer, General Medicine, medicine.disease, Cell culture, 030220 oncology & carcinogenesis, Cancer research, Stem cell, Chondrosarcoma, business

Abstract

For the cancer genomics era, there is a need for clinically annotated close-to-patient cell lines suitable to investigate altered pathways and serve as high-throughput drug-screening platforms. This is particularly important for drug-resistant tumors like chondrosarcoma which has few models available. Here we established and characterized new cell lines derived from two secondary (CDS06 and CDS11) and one dedifferentiated (CDS-17) chondrosarcomas as well as another line derived from a CDS-17-generated xenograft (T-CDS17). These lines displayed cancer stem cell-related and invasive features and were able to initiate subcutaneous and/or orthotopic animal models. Different mutations in Isocitrate Dehydrogenase-1 (IDH1), Isocitrate Dehydrogenase-2 (IDH2), and Tumor Supressor P53 (TP53) and deletion of Cyclin Dependent Kinase Inhibitor 2A (CDKN2A) were detected both in cell lines and tumor samples. In addition, other mutations in TP53 and the amplification of Mouse Double Minute 2 homolog (MDM2) arose during cell culture in CDS17 cells. Whole exome sequencing analysis of CDS17, T-CDS17, and matched patient samples confirmed that cell lines kept the most relevant mutations of the tumor, uncovered new mutations and revealed structural variants that emerged during in vitro/in vivo growth. Altogether, this work expanded the panel of clinically and genetically-annotated chondrosarcoma lines amenable for in vivo studies and cancer stem cell (CSC) characterization. Moreover, it provided clues of the genetic drift of chondrosarcoma cells during the adaptation to grow conditions.

Published

2019

29. Establishment and histopathological study of patient-derived xenograft models and primary cell lines of epithelioid malignant peritoneal mesothelioma.

Author

Yang ZR, Chen ZG, Ji ZH, Lin YL, Zhang J, Ma R, Li Z, Jiang X, Chen Q, Du XM, and Li Y

Subjects

Animals, Disease Models, Animal, Epithelioid Cells pathology, Female, Humans, Male, Mice, Nude, Middle Aged, Cell Line, Tumor pathology, Heterografts pathology, Mesothelioma, Malignant pathology, Mice, Peritoneal Diseases pathology

Abstract

Malignant peritoneal mesothelioma (MPM) is a rare malignancy with few experimental models. This study used the human surgical specimen to establish MPM patient-derived xenograft (PDX) models and primary cell lines to provide a study platform for MPM in vitro and in vivo, and conducted histopathological analysis. Our study used the experimental peritoneal cancer index (ePCI) score to evaluate gross pathology, and the results showed that the ePCI score of the female and male nude mice were 8.80 ± 1.75 and 9.20 ± 1.81 (P=0.6219), respectively. The Hematoxylin and eosin (HE) staining of animal models showed that the tumor was epithelioid mesothelioma and invaded multiple organs. Immunohistochemistry (IHC) staining showed that Calretinin, Cytokeratin 5/6, WT-1 and Ki-67 were all positive. The Swiss-Giemsa and Immunofluorescence (IF) staining of primary cell lines were also consistent with the pathological characteristics of mesothelioma. We also performed the whole-exome sequencing (WES) to identify the mutant genes between models and the patient. And the results showed that 21 mutant genes were shared between the two groups, and the genes related to tumorigenesis and development including BAP1, NF2, MTBP, NECTIN2, CDC23, LRPPRC, TRIM25, and DHRS2. In conclusion, the PDX models and primary cell lines of MPM were successfully established with the epithelioid mesothelioma identity confirmed by histopathological evidence. Moreover, our study has also illustrated the shared genomic profile between models and the patient.

Published

2021

30. Achimota Pararubulavirus 3: A New Bat-Derived Paramyxovirus of the Genus Pararubulavirus .

Author

Baker KS, Tachedjian M, Barr J, Marsh GA, Todd S, Crameri G, Crameri S, Smith I, Holmes CEG, Suu-Ire R, Fernandez-Loras A, Cunningham AA, Wood JLN, and Wang LF

Subjects

Animals, Cells, Cultured, Chlorocebus aethiops, Genome, Viral, Kidney cytology, Kidney virology, Paramyxoviridae Infections urine, Paramyxovirinae isolation & purification, RNA, Viral, Vero Cells, Whole Genome Sequencing, Zoonoses virology, Chiroptera virology, Paramyxoviridae Infections veterinary, Paramyxovirinae classification, Phylogeny

Abstract

Bats are an important source of viral zoonoses, including paramyxoviruses. The paramyxoviral Pararubulavirus genus contains viruses mostly derived from bats that are common, diverse, distributed throughout the Old World, and known to be zoonotic. Here, we describe a new member of the genus Achimota pararubulavirus 3 (AchPV3) and its isolation from the urine of African straw-coloured fruit bats on primary bat kidneys cells. We sequenced and analysed the genome of AchPV3 relative to other Paramyxoviridae , revealing it to be similar to known pararubulaviruses. Phylogenetic analysis of AchPV3 revealed the failure of molecular detection in the urine sample from which AchPV3 was derived and an attachment protein most closely related with AchPV2-a pararubulavirus known to cause cross-species transmission. Together these findings add to the picture of pararubulaviruses, their sources, and variable zoonotic potential, which is key to our understanding of host restriction and spillover of bat-derived paramyxoviruses. AchPV3 represents a novel candidate zoonosis and an important tool for further study., Competing Interests: The authors declare no conflicts of interest.

Published

2020

31. New Chondrosarcoma Cell Lines with Preserved Stem Cell Properties to Study the Genomic Drift During In Vitro/In Vivo Growth.

Author

Rey, Veronica, Menendez, Sofia T., Estupiñan, Oscar, Rodriguez, Aida, Santos, Laura, Tornin, Juan, Martinez-Cruzado, Lucia, Castillo, David, Ordoñez, Gonzalo R., Costilla, Serafin, Alvarez-Fernandez, Carlos, Astudillo, Aurora, Braña, Alejandro, and Rodriguez, Rene

Subjects

*CHONDROSARCOMA, *CELL lines, *STEM cells, *CANCER stem cells, *CELL culture, *GENETIC drift

Abstract

For the cancer genomics era, there is a need for clinically annotated close-to-patient cell lines suitable to investigate altered pathways and serve as high-throughput drug-screening platforms. This is particularly important for drug-resistant tumors like chondrosarcoma which has few models available. Here we established and characterized new cell lines derived from two secondary (CDS06 and CDS11) and one dedifferentiated (CDS-17) chondrosarcomas as well as another line derived from a CDS-17-generated xenograft (T-CDS17). These lines displayed cancer stem cell-related and invasive features and were able to initiate subcutaneous and/or orthotopic animal models. Different mutations in Isocitrate Dehydrogenase-1 (IDH1), Isocitrate Dehydrogenase-2 (IDH2), and Tumor Supressor P53 (TP53) and deletion of Cyclin Dependent Kinase Inhibitor 2A (CDKN2A) were detected both in cell lines and tumor samples. In addition, other mutations in TP53 and the amplification of Mouse Double Minute 2 homolog (MDM2) arose during cell culture in CDS17 cells. Whole exome sequencing analysis of CDS17, T-CDS17, and matched patient samples confirmed that cell lines kept the most relevant mutations of the tumor, uncovered new mutations and revealed structural variants that emerged during in vitro/in vivo growth. Altogether, this work expanded the panel of clinically and genetically-annotated chondrosarcoma lines amenable for in vivo studies and cancer stem cell (CSC) characterization. Moreover, it provided clues of the genetic drift of chondrosarcoma cells during the adaptation to grow conditions. [ABSTRACT FROM AUTHOR]

Published

2019

32. Selective isolation and characterization of primary cells from normal breast and tumors reveal plasticity of adipose derived stem cells

Author

Annika, Weigand, Anja M, Boos, Kereshmeh, Tasbihi, Justus P, Beier, Paul D, Dalton, Michael, Schrauder, Raymund E, Horch, Matthias W, Beckmann, Pamela L, Strissel, and Reiner, Strick

Subjects

Primary cell lines, Cell Plasticity, Primary Cell Culture, Breast Neoplasms, Epithelial Cells, Mesenchymal Stem Cells, Stem cells plasticity, Normal breast, Neoplasm Proteins, Breast cancer, Cell Line, Tumor, Culture Media, Conditioned, Adipocytes, Humans, Female, Tissue engineering, Breast, Mammary Glands, Human, Cell Proliferation, Research Article

Abstract

Background There is a need to establish more cell lines from breast tumors in contrast to immortalized cell lines from metastatic effusions in order to represent the primary tumor and not principally metastatic biology of breast cancer. This investigation describes the simultaneous isolation, characterization, growth and function of primary mammary epithelial cells (MEC), mesenchymal cells (MES) and adipose derived stem cells (ADSC) from four normal breasts, one inflammatory and one triple-negative ductal breast tumors. Methods A total of 17 cell lines were established and gene expression was analyzed for MEC and MES (n = 42) and ADSC (n = 48) and MUC1, pan-KRT, CD90 and GATA-3 by immunofluorescence. DNA fingerprinting to track cell line identity was performed between original primary tissues and isolates. Functional studies included ADSC differentiation, tumor MES and MEC invasion co-cultured with ADSC-conditioned media (CM) and MES adhesion and growth on 3D-printed scaffolds. Results Comparative analysis showed higher gene expression of EPCAM, CD49f, CDH1 and KRTs for normal MEC lines; MES lines e.g. Vimentin, CD10, ACTA2 and MMP9; and ADSC lines e.g. CD105, CD90, CDH2 and CDH11. Compared to the mean of all four normal breast cell lines, both breast tumor cell lines demonstrated significantly lower ADSC marker gene expression, but higher expression of mesenchymal and invasion gene markers like SNAI1 and MMP2. When compared with four normal ADSC differentiated lineages, both tumor ADSC showed impaired osteogenic and chondrogenic but enhanced adipogenic differentiation and endothelial-like structures, possibly due to high PDGFRB and CD34. Addressing a functional role for overproduction of adipocytes, we initiated 3D-invasion studies including different cell types from the same patient. CM from ADSC differentiating into adipocytes induced tumor MEC 3D-invasion via EMT and amoeboid phenotypes. Normal MES breast cells adhered and proliferated on 3D-printed scaffolds containing 20 fibers, but not on 2.5D-printed scaffolds with single fiber layers, important for tissue engineering. Conclusion Expression analyses confirmed successful simultaneous cell isolations of three different phenotypes from normal and tumor primary breast tissues. Our cell culture studies support that breast-tumor environment differentially regulates tumor ADSC plasticity as well as cell invasion and demonstrates applications for regenerative medicine. Electronic supplementary material The online version of this article (doi:10.1186/s13058-016-0688-2) contains supplementary material, which is available to authorized users.

Published

2015

33. Primary cell lines: false representation or model system? a comparison of four human colorectal tumors and their coordinately established cell lines.

Author

Pastor DM, Poritz LS, Olson TL, Kline CL, Harris LR, Koltun WA, Chinchilli VM, and Irby RB

Abstract

Cultured cell lines have played an integral role in the study of tumor biology since the early 1900's. The purpose of this study is to evaluate colorectal cancer (CRC) cell lines with respect to progenitor tumors and assess whether these cells accurately and reliably represent the cancers from which they are derived. Primary cancer cell lines were derived from fresh CRC tissue. Tumorigenicity of cell lines was assessed by subcutaneous injection of cells into athymic mice and calculation of tumor volume after 3 weeks. DNA ploidy was evaluated by flow cytometry. Invasive ability of the lines was tested with the MATRIGEL invasion assay at 24 or 48 hours. Cells were assessed for the presence of Kirsten-Ras (K-Ras), p-53, deleted in colon cancer (DCC), and Src. Protein profiling of cells and tissue was performed by surface enhanced laser desorption/ionization-time of flight/mass spectroscopy. microRNA expression in cell and tumor tissue samples was evaluated by FlexmiR MicroRNA Assays. Four cell lines were generated from tumor tissue from patients with CRC and confirmed to be tumorigenic (mean tumor volume 158.46 mm(3)). Two cell lines were noted to be diploid; two were aneuploid. All cell lines invaded the MATRIGEL starting as early as 24 hours. K-Ras, p53, DCC, and Src expression were markedly different between cell lines and corresponding tissue. Protein profiling yielded weak-to-moderate correlations between cell samples and respective tissues of origin. Weak-to-moderate tau correlations for levels of expression of human microRNAs were found between cells and respective tissue samples for each of the four pairings. Although our primary CRC cell lines vary in their expression of several tumor markers and known microRNAs from their respective progenitor tumor tissue, they do not statistically differ in overall profiles. Characteristics are retained that deem these cell lines appropriate models of disease; however, data acquired through the use of cell culture may not always be a completely reliable representation of tumor activity in vivo.

Published

2010

34. A Method for Prolonged Survival of Primary Cell Lines

Published

2006