Intl Journal of Cancer

2007

DOI: 10.1002/ijc.22925

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Total loss of HLA class I expression on a melanoma cell line after growth in nude mice in absence of autologous antitumor immune response

¹

,

Angel García-Lora

²

,

³

et al.

Abstract: Loss of HLA class I expression on tumor cells is a frequent event as an immune escape mechanism. Seven different altered HLA phenotypes have been defined in tumors. Various molecular mechanisms have been described as responsible for HLA class I loss. HLA class I expression alterations occur successively and unpredictably during tumor progression in vivo and immunoselection has been implicated in this process. We present an experimental xenograft model in which melanoma cell line Ando-2 injected into athymic nu… Show more

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Cited by 12 publications

(17 citation statements)

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“…On the other hand, trichostatin A counteracted HLA down-modulation in IGROV-1 cells, a finding suggesting that histone acetylation may represent an additional relevant mechanism, as previously reported in a different setting [3]. These data are also in line with a previous study reporting an epigenetic effect of the microenvironment, where bystander stromal cells may have a major influence on the growth and progression of tumors [14].…”

Section: Discussionsupporting

confidence: 88%

“…To evaluate this possibility, we cultured tumor cells explanted ex vivo with different epigenetic drugs (namely, trichostatin A and decitabine) that had already proven to be effective in vitro [3, 4] or in vivo [1], respectively. Surprisingly, we observed that the simple placement of tumor cells in complete medium, without the addition of any drug, led to reversion of the down-modulated phenotype (when present) within a few hours (data not shown).…”

Section: Resultsmentioning

confidence: 99%

“…Tumor cells explanted ex vivo were cultured in vitro with different epigenetic drugs (trichostatin A and decitabine, also known as 2′-deoxy-5-azacytidine) that had already proven to be effective in vitro [3, 4] or in vivo [1]. Cells were plated at 5 × 10 5 cells/well in 24-well plate in complete medium (control) or medium added with trichostatin A (50, 250, and 500 nM, Sigma) or decitabine (1 μM, Pharmachemie B.V., Haarlem, Holland), for up to 72 h. For in vivo experiments, mice were treated with trichostatin A (1 mg/kg once a day, days 0–3, Sigma [5]), decitabine (0.25 mg/kg once at day 0, then twice a day, days 1–3 [1]), suberoylanilide hydroxamic acid (SAHA, 1.25 mg/mouse, once a day, days 1–3, Alexis Biochemicals, Lausen, Switzerland [6]), valproic acid (5 mg/mouse, once a day, days 1–3, modified from [7], Sigma), and Interferon-γ (50,000 IU/mouse, once, 6 h before cells recovery, modified from [1], PeproTech, Rocky Hill, NJ).…”

Section: Methodsmentioning

confidence: 99%

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Differential down-modulation of HLA class I and II molecule expression on human tumor cell lines upon in vivo transfer

¹

,

²

,

³

et al. 2011

Cancer Immunol Immunother

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Previous evidence from our laboratory showed that Epstein–Barr virus–immortalized lymphoblastoid B cells undergo a prominent down-modulation of HLA-II molecule expression when injected intraperitoneally in SCID mice, while HLA-I remains almost unaffected. Since this phenomenon can alter the experimental outcome of therapeutic protocols of adoptive cell therapy, we decided to evaluate the behavior of MHC antigens in a panel of cell lines belonging to the B- and T-cell lineages, as well as in epithelial tumor cell lines. Cells were administered in mice either intraperitoneally or subcutaneously and recovered 4 days later for HLA molecule expression analysis. Collected data showed a highly heterogeneous in vivo behavior of the various cell lines, which could alternatively down-modulate, completely abrogate or maintain unchanged the expression of either MHC-I or MHC-II molecules. Moreover, the site of injection impacted differentially on these aspects. Although such phenomena still lack a comprehensive clarification, epigenetic mechanisms are likely to be involved as epigenetic drugs could partially counteract MHC down-modulation in vivo. Nonetheless, it has to be pointed out that careful attention must be paid to the assessment of therapeutic efficacy of translational protocols of adoptive immunotherapy, as modulation of MHC molecules on human target cells when transferred in a mouse environment could readily interfere with the desired and expected therapeutic effects.Electronic supplementary materialThe online version of this article (doi:10.1007/s00262-011-1086-3) contains supplementary material, which is available to authorized users.

“…On the other hand, trichostatin A counteracted HLA down-modulation in IGROV-1 cells, a finding suggesting that histone acetylation may represent an additional relevant mechanism, as previously reported in a different setting [3]. These data are also in line with a previous study reporting an epigenetic effect of the microenvironment, where bystander stromal cells may have a major influence on the growth and progression of tumors [14].…”

Section: Discussionsupporting

confidence: 88%

“…To evaluate this possibility, we cultured tumor cells explanted ex vivo with different epigenetic drugs (namely, trichostatin A and decitabine) that had already proven to be effective in vitro [3, 4] or in vivo [1], respectively. Surprisingly, we observed that the simple placement of tumor cells in complete medium, without the addition of any drug, led to reversion of the down-modulated phenotype (when present) within a few hours (data not shown).…”

Section: Resultsmentioning

confidence: 99%

“…Tumor cells explanted ex vivo were cultured in vitro with different epigenetic drugs (trichostatin A and decitabine, also known as 2′-deoxy-5-azacytidine) that had already proven to be effective in vitro [3, 4] or in vivo [1]. Cells were plated at 5 × 10 5 cells/well in 24-well plate in complete medium (control) or medium added with trichostatin A (50, 250, and 500 nM, Sigma) or decitabine (1 μM, Pharmachemie B.V., Haarlem, Holland), for up to 72 h. For in vivo experiments, mice were treated with trichostatin A (1 mg/kg once a day, days 0–3, Sigma [5]), decitabine (0.25 mg/kg once at day 0, then twice a day, days 1–3 [1]), suberoylanilide hydroxamic acid (SAHA, 1.25 mg/mouse, once a day, days 1–3, Alexis Biochemicals, Lausen, Switzerland [6]), valproic acid (5 mg/mouse, once a day, days 1–3, modified from [7], Sigma), and Interferon-γ (50,000 IU/mouse, once, 6 h before cells recovery, modified from [1], PeproTech, Rocky Hill, NJ).…”

Section: Methodsmentioning

confidence: 99%

See 1 more Smart Citation

Differential down-modulation of HLA class I and II molecule expression on human tumor cell lines upon in vivo transfer

¹

,

²

,

³

et al. 2011

Cancer Immunol Immunother

View full text Add to dashboard Cite

Previous evidence from our laboratory showed that Epstein–Barr virus–immortalized lymphoblastoid B cells undergo a prominent down-modulation of HLA-II molecule expression when injected intraperitoneally in SCID mice, while HLA-I remains almost unaffected. Since this phenomenon can alter the experimental outcome of therapeutic protocols of adoptive cell therapy, we decided to evaluate the behavior of MHC antigens in a panel of cell lines belonging to the B- and T-cell lineages, as well as in epithelial tumor cell lines. Cells were administered in mice either intraperitoneally or subcutaneously and recovered 4 days later for HLA molecule expression analysis. Collected data showed a highly heterogeneous in vivo behavior of the various cell lines, which could alternatively down-modulate, completely abrogate or maintain unchanged the expression of either MHC-I or MHC-II molecules. Moreover, the site of injection impacted differentially on these aspects. Although such phenomena still lack a comprehensive clarification, epigenetic mechanisms are likely to be involved as epigenetic drugs could partially counteract MHC down-modulation in vivo. Nonetheless, it has to be pointed out that careful attention must be paid to the assessment of therapeutic efficacy of translational protocols of adoptive immunotherapy, as modulation of MHC molecules on human target cells when transferred in a mouse environment could readily interfere with the desired and expected therapeutic effects.Electronic supplementary materialThe online version of this article (doi:10.1007/s00262-011-1086-3) contains supplementary material, which is available to authorized users.

“…We constructed both vectors carrying HLA-A2 gene and compared their efficacy to induce HLA-A2 transgene expression in different tumor cell lines. Using these viral vectors, we successfully recovered HLA-A2 expression in melanoma cell line Ando-2 which has been characterized to lack endogenous HLA-A2 due to a haplotype loss caused by loss of heterozygosity at chromosome 6 (Table 1) [26]. (Table 1).…”

Section: Comparative Analysis Of the Transduction Efficacy Of Adenovimentioning

confidence: 99%

“…All melanoma cell lines, except for Ando-2, were obtained from the European Searchable Tumour Cell Line Data Base (ESTDAB) [24] and have been previously genotyped for HLA-I and characterized for HLA phenotype [25]. Ando-2 was kindly provided by Dr P. Coulie (Université Catholique de Louvain (UCL), Brussels, Belgium) and is characterized by the loss of HLA-A2 expression due to HLA-I haplotype loss [26]. Prostate cancer cell lines DU145 and PC3, as well as bladder cancer cell lines T24, WIL and RT112, were obtained from American Type Culture Collection (ATCC).…”

Section: Cell Linesmentioning

confidence: 99%

Recovery HLA-A2 and Beta2-microglobulin Expression in Tumor Cells Using Viral Vectors

Fj¹,

A²,

et al. 2017

J Cancer Sci Ther

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Background: Tumor elimination and the success of cancer immunotherapy depend on the proper expression of HLA class I complex (HLA-I) required for the presentation of tumor-associated peptides to cytotoxic T-lymphocytes. Tumors escape immune attack by losing HLA-I expression, often due to irreversible genetic/chromosomal alterations, including mutations in beta2-microglobulin (B2M) or lack of HLA-A2 allele due to a haplotype loss. The introduction of these genes and re-expression of the missing HLA-I specificity on the tumor cell surface is an attractive strategy to induce tumor rejection by T-lymphocytes. Methods:Using genomic HLA-I typing and gene sequencing we determined HLA-I phenotypes and alterations in different human tumor cell lines previously characterized in our laboratory. We used adeno-and adeno-associated viruses to reconstitute/up-regulate HLA-A2 or/and B2M expression in these cells in vitro. Using flow cytometry and immunocytochemistry we evaluated levels and patterns of HLA-I expression in these cells. Results:We have defined altered HLA-I genotypes in various human tumor cell lines. Ad5 and, to a lesser degree, AAV2 vectors were efficient in a replacement of mutated B2M, recovery of lost endogenous HLA-A2 allele, and de novo expression of an additional HLA-A2 allele in tumor cells naturally lacking HLA-A2. Ad5-mediated co-transfection of both HLA-A2 and B2M demonstrated that the de novo expressed proteins associate to form a detectable HLA-I/B2M complex on the cell surface. Conclusion:Using gene therapy, it is possible to recover normal B2M and HLA-A2 gene expression caused by structural "hard" alteration and to induce co-expression of both genes in cells naturally lacking HLA-A2 allele. In addition, we demonstrated that transfected tumor cells are able to express seven HLA-I alleles. The recovery of the missing HLA-I molecules in tumor cells using adeno and adeno-associated viruses can be a useful strategy to circumvent cancer immune escape and increase tumor rejection.

The tumour suppressor Fhit positively regulates MHC class I expression on cancer cells

¹

,

³

et al. 2012

The Journal of Pathology

Self Cite

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MHC class I (MHC‐I) molecules are ubiquitously expressed on the cells of an organism. Study of the regulation of these molecules in normal and disease conditions is important. In tumour cells, the expression of MHC‐I molecules is very frequently lost, allowing these cells to evade the immune response. Cancers of different histology have shown total loss of MHC‐I molecule expression, due to a coordinated transcriptional down‐regulation of various antigen‐processing machinery (APM) components and/or MHC‐I heavy chains. The mechanisms responsible for these alterations remain unclear. We determined the possible genes involved by comparing MHC‐I‐positive with MHC‐I‐negative murine metastases derived from the same fibrosarcoma tumour clone. MHC‐I‐negative metastases showed transcriptional down‐regulation of APM and MHC‐I heavy chains. The use of microarrays and subtraction cDNA libraries revealed four candidate genes responsible for this alteration, but two of them were ruled out by real‐time RT‐PCR analyses. The other two genes, AP‐2α and Fhit tumour suppressors, were studied by using siRNA to silence their expression in a MHC‐I‐positive metastatic cell line. AP‐2α inhibition did not modify transcriptional expression of APM components or MHC‐I heavy chains or surface expression of MHC‐I. In contrast, silencing of the Fhit gene produced the transcriptional down‐regulation of APM components and MHC‐I heavy chains and decreased MHC‐I surface expression. Moreover, transfection of Fhit in MHC‐I‐negative tumour cell lines restored MHC‐I cell surface expression. These data indicate that defects in Fhit expression may promote MHC‐I down‐regulation in cancer cells and allow escape from immunosurveillance#. Copyright © 2012 Pathological Society of Great Britain and Ireland. Published by John Wiley & Sons, Ltd.

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