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Authenticating Cell Lines in Ophthalmic Research Laboratories

¹From Oakland University William Beaumont School of Medicine, Rochester, Michigan; the ²Department of Pathology, University of Illinois at Chicago, Chicago, Illinois; the ³Department of Ophthalmology, Leiden University Medical Centre, Leiden, the Netherlands; and the ⁴Department of Ophthalmology, Hadassah-Hebrew University Medical, Jerusalem, Israel.

Authentication of cell lines in biomedical research has been elevated to a very high priority. In a review of the literature, Lacroix¹ examined the issue of cross-contamination of cell lines including the well-known contamination of cell lines with HeLa cells,² and the misidentification of the ECV304 cell line as "immortalized endothelial cells" when these cells in fact originated from T24 bladder carcinoma cells.³ Lacroix¹ estimated that between 18% and 36% of cell lines have been misclassified. One survey at a large research institution suggested that fewer than 50% of researchers authenticate their cell lines.⁴ Nardone⁵ proposed recently that identification of cell lines be required of investigators before grants are awarded, and the National Institutes of Health subsequently called for researchers to authenticate cell lines as a prerequisite for grant funding.⁶

Cell lines are widely used in ophthalmic investigations. The authors’ own research efforts have been focused on the biology of metastasis of uveal melanoma, and in the field of ocular oncology research, the use of cell lines is critical for at least two reasons. First, there are no animal models of spontaneous uveal melanoma that faithfully replicate the behavior of the human disease.⁷ Transgenic models of uveal melanoma do not reproduce histogenesis of human uveal melanoma, and spontaneous uveal melanomas develop too sporadically in nature to be valuable in research,^{8 9 10 11 12 13} or the animal melanoma tumors vary significantly from their human counterparts.¹⁴ Therefore, uveal melanoma researchers have increasingly relied on the implantation of animal and human melanoma cell lines into animals to model the behavior of human uveal melanoma to improve imaging techniques^{15 16 17} and to investigate immunologic^{18 19} and molecular mechanisms of tumor behavior.^{20 21}

Second, mindful of the reality that statistical associations between histologic characteristics and outcome do not always indicate causality, the availability of cell lines allows ophthalmic researchers to advance from correlative studies to mechanistic investigations using advanced molecular methodologies. For example, All-Ericsson et al.²² identified the association between the expression of insulin-like growth factor-1 by immunohistochemistry in tissue sections of uveal melanoma and adverse outcome and also demonstrated decreased tumor cell viability in uveal melanoma cell lines after interfering with the expression of ILGRF-1, pointing to the molecular significance of this histologic finding. Later, Girnita et al.,²¹ from the same group, expanded on this finding to suggest a novel therapeutic approach to uveal melanoma using the pharmacological manipulation of ILGRF-1 in human uveal melanoma cell lines.

It is possible that the behavior of long-term cell lines is not representative of the spectrum of phenotypic behavior of neoplasms, because those lines that are established in vitro have been selected for this artificial growth environment. In addition, the phenotypic behavior of cancer cell lines can change over time. And yet, despite these limitations, there are few satisfactory alternatives to the use of long-term cell lines in modeling uveal melanoma behavior in animals or testing molecular approaches to the modifying of tumor cell behavior. Some investigators have preferred to work with short-term primary cultures to circumvent these limitations of long-term cell lines, but short-term cultures cannot be reliably shared between investigative groups, making it difficult to obtain independent validation of results on common biological substrates. Therefore, investigators have developed mechanisms for sharing long-term cell lines between groups.

In many areas of biomedical research, investigators obtain long-term cell lines from centralized repositories. However, many cell lines developed for ophthalmic research are not available from these agencies. For example, uveal melanoma cell lines are not identified in the inventories of the American Tissue Culture Collection (ATCC, Manassas, VA, www.atcc.org), the Deutsche Sammlung von Mikroorganismen und Zellkulturen (DSMZ; Braunschweig, Germany; www.dsmz.de), the European Collection of Cell Cultures (ECACC; www.ecacc.org.uk), or the Japanese Collection of Research Bioresources (JCRB; Osaka, Japan; http://cellbank.nibio.go.jp). The European Molecular Biology Laboratory-European Bioinformatics Institute (EMBL-EBI; Cambridge, UK) Web site (http://www.ebi.ac.uk/ipd/estdab/directory.html) lists only four uveal melanoma cell lines: OCM3, OCM8, 92.1, and Mel-202. To complicate matters, it is relatively difficult to establish new long-term uveal melanoma cell lines. One investigator noted that more than 60% of attempts to establish such lines were unsuccessful.²³ Therefore, as in the case of many ophthalmic research endeavors, ophthalmic oncology researchers have shared uveal melanoma cell lines with each other.

The relatively few uveal melanoma cell lines available for research have been widely circulated, but it is clear from scanning the methods sections of publications in this field that the source of the cell line does not always represent the investigator who actually developed the cell line, indicating the existence of secondary and even tertiary distributions of these scarce but vital resources. The underlying assumption behind this collegial sharing of resources is simple: A named cell line used in the United States is identical with the cell line being used in Europe or Asia with the same name. One also assumes that human lines are indeed human. We are aware of the practice of propagating uveal melanoma cell lines in immunosuppressed mice, introducing the risk that murine cells may contaminate cultures or that murine pathogens can infect cultures and, at least theoretically, alter the phenotypic behavior of the tumor cells. In addition, several of the authors (MJJ, KVN, AJM, RF) have discovered that cell lines in their laboratories that were presumed to be human were in fact murine. In each case, rigorous quality control procedures in the laboratories identified the lines as nonhuman, and no data were ever published by any of the authors using murine cell lines that were presumed to be human. Nevertheless, these experiences highlight the need to maintain vigilance in authenticating presumed human cell lines as indeed human.

In our own research, we have used several long-term uveal melanoma cell lines that have been distributed widely by the laboratories that first developed them. The OCM1, OCM3, OCM8, C918, M619, MUM2B, and MUM2C cell lines were obtained by our laboratory between 2000 and 2007 as gifts from the laboratories in which these cell lines originated. We recently became aware of the misidentification of some of these lines. Our laboratory was interested in identifying novel BRAF mutations in uveal melanoma cell lines. It has already been shown that the OCM1 cell line was positive for the V599E mutation,^{24 25} a finding of interest because, in contrast with cutaneous melanoma²⁶ and conjunctival melanomas,^{27 28} the V599E (also known as V600E) mutation is not commonly found in uveal melanomas except for those tumors originating in the iris.²⁹ Recently, Maat et al.³⁰ identified the V600E mutation in OCM1 and OCM3, and we confirmed the V599E mutation in the OCM1 and OCM3 cell lines and determined that the M619, C918, and MUM2B cell lines were negative for this mutation. We were surprised to discover that the MUM2C cell line was also positive for the V599E mutation, because according to the literature, the MUM2B and MUM2C cell lines were cloned from cells originating in a single hepatic metastasis.³¹ This led us to question whether MUM2B and MUM2C were truly syngeneic.

	The Misidentification of Uveal Melanoma Cell Lines

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The OCM cell lines have been described extensively in the literature as originating from primary uveal melanomas.³² The C918 and M619 cell lines were also developed from primary uveal melanomas.³³ The MUM cell lines were reported to have originated from a hepatic metastasis of a uveal melanoma.³¹ Each cell line was characterized by immunohistochemistry (S100 protein, HMB45, and Melan-A) and the ability to generate vasculogenic mimicry patterns in three-dimensional cultures.³¹

In performing internal quality controls on our lines, we validated the absence of human pathogens: Mycoplasma species, hepatitis B virus (HBV), hepatitis C virus (HCV), and human immunodeficiency virus (HIV) I and II by PCR-based tests performed at Charles River Diagnostics (Mycoplasma) (Wilmington, MA), Clongen Laboratories (HBV, HCV, HIV) (Germantown, MD), and the University of Illinois at Chicago, Department of Pathology, Molecular Genetics Laboratory (HBV, HCV, HIV). All cell lines were also negative for 13 murine viral pathogens, including mouse parvoviruses MPV-1 and -2, minute virus of mice, mouse hepatitis virus, reovirus types 1 and 3, lymphocytic choriomeningitis virus, lactate dehydrogenase-elevating virus, mouse rotavirus, Theiler’s murine encephalomyelitis virus, mousepox, hantavirus Hantaan, and hantavirus Seoul (Mouse Essential Panel, Fluorogenic PCR Infectious Agent Assays; Charles River Diagnostics).

Karyotypes were analyzed by growing cells in standard conditions in RPMI-1640, followed by harvesting and G banding according to standard methods. Eight to 22 cells were analyzed for each cell line, and karyotypes were described according to the ISCN 2005 nomenclature. Genomic DNA was extracted from each cell line with a cell and tissue kit (Puregene; Qiagen, Valencia, CA) according to the manufacturer’s protocol. DNA purity and concentration were measured spectrophotometrically. Genetic identity was determined by short tandem repeat (STR) analysis (Profiler Plus and COfiler kits; Applied Biosystems, Inc. [ABI], Foster City, CA) according to the manufacturer’s protocol. Amplicons were generated by multiplex PCR and electrophoresed on a genetic analyzer (model 3100; ABI). The data were then analyzed (GeneMapper 4.0 software; ABI).

The OCM cell lines are no longer available from the originator³² of these cells. For the authentication of all other cell lines, we obtained original stocks of C918 and M619 dated 1996, and compared the STR profiles of these cells with those provided to us between 2000 and 2007. We also compared STR profiles of the MUM cells provided to us by the originating laboratory with the original stocks. For each of these cell lines, we detected no differences between the STR profiles of the original stocks, cells provided to us by the donor laboratory, and cells currently in use in our laboratory.

The STR profiles for the cell lines tested, summarized in Table 1 , indicate that OCM1 and MUM2C are from the same patient, and that M619, C918, and MUM2B are from the same patient. Historically, the MUM2B cell line has been described as originating from the liver of a patient with metastatic uveal melanoma who eventually died of the disease. We therefore obtained archival tissue from this patient’s biopsy sample on file in the laboratory that provided the cells to us, extracted genomic DNA from the tissues, and compared STR profiles between this patient who died of metastatic uveal melanoma and MUM2B cells. These analyses indicate that cells designated as MUM2B are not genetically related to the patient who died of metastatic uveal melanoma. The C918 and M619 cell lines were historically derived from primary uveal melanomas. We therefore conclude that the MUM2B cell line—from the same patient as C918 and M619—is derived from a primary and not a metastatic uveal melanoma. We were able to extract genomic DNA from paraffin-embedded samples of the tumor from which M619 was derived, and the STR profile of this tumor did not match the common STR profiles of M619, C918, or MUM2B cells. We have not been able to obtain tissue from the patient’s tumor sample from which C918 was developed, but we believe that it is reasonable to infer that MUM2B, C918, and M619 are all derived from the tumor that gave rise to C918.

There are subtle differences in immunohistochemical profiles, even among cell lines that are genetically identical according to STR analyses (Table 1) . We also noticed changes in the immunohistochemical expression of melanoma markers over time. For example, the staining for S100 protein is more intense in the MUM2B cells obtained from the donor laboratory than in the same cells after at least 10 passages in our own laboratory, whereas the STR profiles of the MUM2B cells before and after passaging in our laboratory remained constant, indicating a phenotypic drift. Variations in karyotypic analyses were also detected between cell lines with identical STR profiles (Table 2 compares the karyotypes of M619 and C918), and similar to our experience with immunohistochemistry, subtle changes in the karyotypic profiles were detected after passaging, whereas STR profiles of these cell lines did not change after passaging in our laboratory.

	Implications for the Uveal Melanoma Research Community

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With only two exceptions, the publications from our group that used these cell lines dealt with phenotypic behavior (Barak V, et al. IOVS 2007;48:ARVO E-Abstract 1947).^{35 36 37 38 39 40 41 42} The conclusions of these papers are therefore still valid in the context of comparing the behavior of invasive/aggressive uveal melanoma cells and noninvasive/poorly aggressive uveal melanoma cells. In one study, we compared gene expression between MUM2B (C918) and MUM2C (OCM1)—valid comparisons between a highly invasive/aggressive cell line (C918) and a poorly invasive/aggressive cell line (OCM1).³⁶ In another study, we compared gene expression between two highly invasive cell lines (M619 and MUM2B) and a poorly invasive/aggressive cell line (OCM1), but even this comparison is valid, because the comparisons were made between two phenotypic variants of the same highly invasive/aggressive uveal melanoma cell line (C918) as defined by identical STR profiles and a poorly invasive uveal melanoma cell line (OCM1) with a different STR profile.³⁸

	Implications and Recommendations for the General Vision Research Community

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Although the incident we describe in this communication came to light in the domain of uveal melanoma research, the imperative of authenticating cell lines extends to all disciplines within the vision research community. It is important that vision researchers using cell lines authenticate their lines against a published standard; assure journal editors, journal readers, and granting agencies that their cell lines have been authenticated; and take measures to eliminate the risks of cell line cross-contamination in their laboratories.

The requirement for investigators to authenticate their cell lines against a standard necessitates a central repository of either cell lines or data by which cell lines can be authenticated. Although investigators funded by the National Institutes of Health are expected to share their cell lines with those who request these resources, it may not serve the interests of the vision research community to require that the cell lines be deposited physically with a central repository such as the ATCC. The number of ophthalmic investigators using a cell line of interest is limited compared with the number of investigators who use cell lines typically stocked in centralized repositories. Moreover, the withdrawal of cell lines from repositories is associated with a fee, thus limiting access to these cells to investigators of limited financial means.

In our investigations, we relied on STR methodology to characterize the uveal melanoma cell lines for the reasons summarized recently by Josephson et al.⁴³ : (1) STR analysis is a simple, relatively inexpensive test available in kit form from several vendors; (2) STR analysis readily identifies male and female samples; (3) STR analysis permits the discrimination of fewer than 1 in 10⁸ individuals⁴⁴ ; and (4) STR analysis is now used as an authentication benchmark by central cell line repositories. The ATTC now provides a comprehensive STR database for cell lines and encourages investigators to fingerprint cells in their laboratories and to compare the analyses against the information published and available online (http://www.atcc.org/CulturesandProducts/CellBiology/STRProfileDatabase/tabid/174/Default.aspx). The ECACC uses a combination of methods to authenticate cell lines including isoenzyme analysis, multilocus DNA fingerprinting, and STR profiling (http://www.ecacc.org.uk/). The DSMZ provides investigators with information on cell lines in their repository, including cytogenetics, DNA typing (STR profiling), and immunophenotyping, in addition to speciation and mycoplasma detection and viral analyses (http://www.dsmz.de/human_and_animal_cell_lines/main.php?contentleft_id=21).

Although STR profiling is now emerging as a standard for cell line authentication, other data are useful for investigators. The EMBL-EBI lists STR profiles along with many genomic and molecular profiles including high-resolution HLA typing and HLA and related genes surface expression. The publication by de Waard-Sibienga et al.⁴⁵ in 1995 is an example of a thorough description of a novel uveal melanoma cell line in which the authors provide detailed analyses of HLA profiles. Because of the considerable interest in uveal melanoma immunology, the HLA profiles of novel cell lines, if known, should be shared with the research community.

Requiring investigators to deposit STR analyses into a centralized data repository that can be accessed anonymously by the research community follows the precedent of requiring investigators to post gene expression profiles to centralized data warehouses. In general, it is not sufficient that investigators make STR profiles available on their laboratory Web sites for several reasons: (1) investigators may move from one organization to another, creating orphan links to critical STR profile data; (2) Web sites themselves may not be maintained optimally, resulting in outdated links that do not provide data access; and (3) it is possible for investigators to identify those individuals who seek data about STR profiles from laboratory-maintained Web sites. The creation of a Web-based centralized cell authentication data repository by an "honest broker" would allow for anonymous access of information of importance to the vision research community. Because the number of cell lines of interest to the vision research community is relatively limited, organizations such as ARVO may wish to consider methods by which such a data repository can be constructed and maintained. If the STRs of cell lines were available, then it would be reasonable to require that researchers periodically validate the authenticity of the lines in their laboratories.

It is also reasonable to require that authors declare in papers submitted for publication that cell lines used in their studies (1) have been validated as to species (i.e., the cells are human and not murine if the subject of the investigation is the behavior of human cells), (2) have been validated as pathogen-free, and (3) have been authenticated by STR analysis, if human, against a benchmark standard; and that (4) the investigators follow standard operating procedures including the implementation of quality management programs. This declaration should be no more burdensome than requiring investigators who enroll human subjects or animals in their studies to state that their research conforms to the Declaration of Helsinki or the ARVO policy on using animals in research.

If research laboratories followed the same set of standard operating procedures required of clinical diagnostic laboratories that use human cell lines—such as diagnostic cytogenetics laboratories where the risk of cell line cross-contamination would result in misdiagnoses of horrific proportions—then it is likely that the integrity of cell lines in research laboratories would be improved significantly.⁴⁶ Again, organizations such as ARVO can assume a leadership role in developing and publishing standard operating procedures and quality management programs for investigators who use cell lines.

Dealing with the consequences of cross-contaminated cell lines is wasteful of time and dwindling research resources. The vision research community is now challenged to design and implement strategies to reduce the risk of misidentified cell lines in ophthalmic research.

	Footnotes

 
Supported by National Eye Institute Grant R01-EY10457.

Submitted for publication May 22, 2008; revised June 25, 2008; accepted September 11, 2008.

Disclosure: R. Folberg, None; S.S. Kadkol, None; S. Frenkel, None; K. Valyi-Nagy, None; M.J. Jager, None; J. Pe'er, None; A.J. Maniotis, None

Corresponding author: Robert Folberg, Oakland University William Beaumont School of Medicine, 478 O'Dowd Hall, 2200 N. Squirrel Road, Rochester, MI 48309-4401; rfolberg{at}oakland.edu.

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