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Journal of Ovarian Research logoLink to Journal of Ovarian Research
. 2014 Jun 7;7:60. doi: 10.1186/1757-2215-7-60

Reliable in vitro studies require appropriate ovarian cancer cell lines

Francis Jacob 1,2, Sheri Nixdorf 1, Neville F Hacker 3, Viola A Heinzelmann-Schwarz 1,2,3,
PMCID: PMC4058698  PMID: 24936210

Abstract

Ovarian cancer is the fifth most common cause of cancer death in women and the leading cause of death from gynaecological malignancies. Of the 75% women diagnosed with locally advanced or disseminated disease, only 30% will survive five years following treatment. This poor prognosis is due to the following reasons: limited understanding of the tumor origin, unclear initiating events and early developmental stages of ovarian cancer, lack of reliable ovarian cancer-specific biomarkers, and drug resistance in advanced cases. In the past, in vitro studies using cell line models have been an invaluable tool for basic, discovery-driven cancer research. However, numerous issues including misidentification and cross-contamination of cell lines have hindered research efforts. In this study we examined all ovarian cancer cell lines available from cell banks. Hereby, we identified inconsistencies in the reporting, difficulties in the identification of cell origin or clinical data of the donor patients, restricted ethnic and histological type representation, and a lack of tubal and peritoneal cancer cell lines. We recommend that all cell lines should be distributed via official cell banks only with strict guidelines regarding the minimal available information required to improve the quality of ovarian cancer research in future.

Keywords: Epithelial ovarian cancer, Tubal cancer, Peritoneal cancer, Primary cultures, Immortalization

Introduction

Epithelial ovarian cancer (EOC) is the fifth most common cause of cancer death in women and the leading cause of death from gynaecological malignancies [1]. Survival rates have changed little since the early 1980’s despite the use of new chemotherapeutical drugs, with only 40% of all stages and 15-30% of patients with widespread metastatic disease surviving 5 years after the initial treatment [2]. This poor overall prognosis is the result of a combination of factors including a lack of distinctive symptoms and sensitive/specific tumour markers at an early stage, drug resistance for advanced disease, and a limited understanding of the early-initiating events and early stages of EOC development.

The dualistic paradigm

Among the different tumours arising from the ovary 90% are of epithelial origin [3]. The major histotypes (serous, endometrioid, mucinous, and clear cell) are partly genetically distinguishable as shown by various high-throughput studies in the past fifteen years [4]. Recent findings suggest that epithelial tumours of the ovary may be grouped on the basis of their genetic alterations into a dualistic model that subdivides the various histological types of EOC into two broad categories. The slowly developing tumours (Type I) include low grade serous, endometrioid, mucinous, and a subset of clear cell carcinomas [5-7] and are characterised by genetic alterations in KRAS, BRAF, CTNNB1, PTEN, ARID1A, FBXW74, PIK3CA, PPP2R1A, and TGFBR2[7-12]. The more aggressive Type II tumours harbour mutations in TP53, BRCA1, and BRCA2[8]. A more systematic characterization of Type II tumours, in particular high grade serous ovarian cancers, was performed by The Cancer Genome Atlas (TCGA). The Profiling of 489 samples for differential mRNA and miRNA expression, DNA copy number changes, promoter DNA methylation, and whole exome DNA sequencing revealed that almost all samples comprised TP53 mutations and significantly recurring somatic mutations in NF1, BRCA1, BRCA2, RB1, and CDK12[13].

Ovarian surface epithelium and tubal epithelium as possible tumour origins

The monolayer of epithelial cells covering the outer surface of the ovary (OSE) has traditionally been thought to be the site of origin of epithelial ovarian cancer [1]. This is supported by a recent study focusing on a stem cell niche located at the hilum region and a transitional area between OSE, mesothelium and tubal epithelium. In a comprehensive experimental mouse model the authors demonstrate that stem cell-like OSE cells have the potential to develop into EOC [14]. Another theory proposes the normal epithelium of the fallopian tube (serous), endometrium (endometrioid) and endocervix (mucinous) as the origin of the respective EOC histotypes [15,16]. According to the concept of extra-uterine Müllerian epithelium, the fallopian tube fimbria is proposed to be the primary origin of the high grade serous ovarian carcinoma, the most common EOC subtype and frequently harbouring TP53 and IL-6 mutations [17,18]. This is supported by the presence of early neoplastic serous tubal intraepithelial lesions (STIL) in prophylactically removed fallopian tubes of BRCA mutations-carrying women [19-21]. Those tubal fimbria displayed characteristic features such as TP53 mutations, DNA damage, and secretory cells, suggesting the tubal fimbria as the precursor for high grade serous ovarian cancers [20,22,23]. This was further supported by more recent studies identifying the tubal secretory cells as potential neoplastic precursors at the tubal fimbria. These cells carry TP53 mutations, show elevated γH2AX expression, a marker of DNA damage, and express Ki-67 and PAX2, two proliferation markers also expressed in serous tubal intraepithelial carcinomas and high grade serous ovarian carcinomas [24-27]. In contrast, epithelial-specific marker such as Calretinin and PAX8 do not seem suitable in the proof of EOC origin [28]. Recently, it has been demonstrated in a Brca, Tp53, Pten genetic mouse model that de novo high grade serous ovarian carcinoma are originated from the fallopian tube secretory epithelium and that these tumours are correlated with high grade serous carcinoma tumour markers and genomic alterations of the human TCGA data set [29].

Serous carcinomas of the ovary, tube and peritoneum

Serous ovarian- (SOC), tubal- (STC), and peritoneal- (SPC) cancers are remarkably similar in term of morphology [30,31], genetics [32], and clinical behaviour and epidemiology [33]. SPC and SOC patients also have a comparable survival rate that, however, is markedly distinct from that of patients with low grade SOC metastasizing to distant locations. Cell lines have long been considered important and useful in vitro models to investigate the molecular nature and the pathological processes underlying the development of ovarian, tubal, and peritoneal tumours, and their progression to advanced diseases, and even to search for diagnostic or prognostic tumour markers as well as for therapeutic targets.

Ovarian cancer cell lines need better characterization

Falling short of the use of in vivo animal models, cancer cell lines as in vitro models have proven invaluable experimental tools for many decades in basic research. Cancer cell lines can be grown continuously in culture, allowing countless experiments to be performed without the necessary restrictions required for in vivo models. However, due to few regulations for the development and testing of these cell lines, the question arises as to the quality of long-time established ovarian cancer cell lines. Often laboratories obtain cell lines from collaborating groups and trust in their identification of cells. Conducting research on the basis of such cell lines means not only a waste of a great deal of money and time but also a risk to steer research in an undesired direction.

It is therefore of great importance to define and establish a world-wide standard applicable to all cell lines that are commercially available for research, in order to ensure that only high-quality cancer cell lines with an unequivocal molecular identity and source are distributed to the research community.

We performed a web search for currently available banks for cells and cell lines using the terms ‘cell bank’, ‘cell lines’, and ‘cell line bank’. Only web pages in English and containing normal or cancer ovarian, tubal, and peritoneal cell lines were included in the study. PubMed (http://www.ncbi.nlm.nih.gov/) was also searched to retrieve references provided by these cell banks reporting additional details of the stocked cell lines. We also included a recent publication in which the copy-number changes, mutations, and mRNA expression profiles in ovarian cancer cell lines were compared to those of high grade SOC (TCGA, http://cancergenome.nih.gov/) [34].

Commercially available ovarian cancer cell lines

Five cell banks worldwide that stock and distribute normal and/or ovarian cancer cell lines were identified. These are the American Type Culture Collection (ATCC), the European Collection of Cell Cultures (ECACC), the German Collection of Microorganisms and Cell Cultures (DSMZ), the Japanese Collection of Research Bioresources (JCRB), and the National Cell Bank of Iran (NCBI) (Table  1). Remarkably, the Australian cell bank (Cell Bank Australia) does not stock ovarian cell lines.

Table 1.

Ovarian cancer cell line banks

ID Name Homepage
ATCC
American Type Culture Collection
http://www.lgcstandards-atcc.org
ECACC
European Collection of Cell Cultures, a part of the Health Protection Agency
http://www.phe-culturecollections.org.uk/collections/ecacc.aspx
DSMZ
German Collection of Microorganisms and Cell Cultures
http://www.dsmz.de/
JCRB
Japanese Collection of Research Bioresources
http://cellbank.nibio.go.jp/
CellBank Australia
Australian cell bank – Cell Bank Australia
http://www.cellbankaustralia.com/
NCBI National Cell Bank of Iran http://ncbi.pasteur.ac.ir/

Our search algorithm retrieved 153 cell lines. ECAAC distributes almost 40% of all publicly available cell lines, followed by JCRB (19%). A number of cell lines (7.2%) are distributed by two or more cell banks. A listing of the ID number, cell line designation (name), origin, and source of the retrieved normal and malignant ovarian, tubal, and peritoneal cell lines is presented in Tables  2 and 3. About two thirds (68.0%) of the normal and ovarian cancer cell lines used in research is of human and about one fourth (23.5%) of Chinese hamster (Cricetulus griseus) origin. About 3% originate from mice (Mus musculus) and 4.5% from various species such as Spodoptera frugiperda (Fall armyworm), Esox lucius (Northern pike fish), Ictalurus punctatus (Channel catfish), and Sus domesticus (Domestic pig). Strikingly, one third of the 104 described human ovarian cancer-derived cell lines were in reality not from ovarian tissue but from peritoneal ascites (21.2%), pleural fluid (3.8%), or metastatic masses (6.7%).

Table 2.

Human cell lines originated from ovarian cancer or human ovarian surface epithelium

ID number
Cell line
Origin
Source
Homo sapiens – human
1
222
 
 
2
2008
Ovary
 
3
2008/C13.R
Ovarian adenocarcinoma
NCBI
4
41Ma/OAW28
Ovarian cancer ascites
ECACC
5
41 M cisR
Ovarian cancer ascites
 
6
59 M
Ovarian cancer ascites
ECACC
7
A2780
Ovarian adenocarcinoma
ECACC
8
A2780ADR
Ovarian adenocarcinoma; A2780
ECACC
9
A2780cis
Ovarian adenocarcinoma; A2780
ECACC
10
A2780 CP
Ovarian adenocarcinoma
NCBI
11
A2780 S
Ovarian adenocarcinoma
NCBI
12
Caov-3
Ovarian adenocarcinoma
ATCC
13
Caov-4
Metastatic fallopian tube mass from ovarian tumour
ATCC/NCBI
14
CH1
Ovarian adenocarcinoma
 
15
CH1cisR
Ovarian adenocarcinoma
 
16
COLO-704
Metastatic colonic ascites from ovarian tumour
DSMZ
17
COV318
Ovarian cancer ascites
ECACC
18
COV362
Ovarian cancer pleural effusion
ECACC
19
COV362.4
Ovarian cancer pleural effusion; COV362
ECACC
20
COV413A
Metastatic sigmoid mass from ovarian tumour
ECACC
21
COV413B
Metastatic bladder dome mass from ovarian tumour
ECACC
22
COV434
Ovarian granulosa tumour from a solid primary tumour
ECACC
23
COV504
Ovarian pleural effusion
ECACC
24
COV644
Ovarian cancer (primary tumor)
ECACC
25
EFO-21
Ovarian cancer ascites
DSMZ
26
EFO27
Metastatic omental mass from ovarian tumour
DSMZ
27
ES-2
Ovarian adenocarcinoma
ATCC
28
FU-OV-1
Malignant ovarian mass
DSMZ
29
HAC-2
Ovarian cancer cell derived from mesonephros
JCRB
30
Hey-A8
Ovary
CCLE
31
HOSE 6-3
Ovarian surface epithelium
 
32
HOSE 17-1
Ovarian surface epithelium
 
33
HOSE 105
Ovarian surface epithelium
 
34
HOSE 111
Ovarian surface epithelium
 
35
HOSE 129
Ovarian surface epithelium
 
36
HOSE 130
Ovarian surface epithelium
 
37
Hs 38.T
Ovarian teratoma
ATCC
38
Hs 571.T
Ovarian adenocarcinoma
ATCC
39
Hs904.T
 
 
40
IGROV1
Ovarian adenocarcinoma
 
41
JHOC-5
Ovarian adenocarcinoma
CCLE
42
JHOM-1
Ovarian adenocarcinoma
CCLE
43
JHOM-2B
Ovarian adenocarcinoma
CCLE
44
JHOS-2
Ovarian adenocarcinoma
CCLE
45
JHOS-4
Ovarian adenocarcinoma
CCLE
46
KURAMOCHI
Ovarian cancer ascites
JCRB
47
MCAS
Ovarian adenocarcinoma
JCRB
48
NCC-OvC-K119
Ovarian adenocarcinoma
JCRB
49
OAW28/41 M
Ovarian cancer ascites
ECACC
50
OAW42
Ovarian cancer ascites
ECACC
51
OC 314
Ovarian cancer ascites
CCLE
52
OC 315
Ovarian adenocarcinoma
CCLE
53
OC 316
Ovarian cancer ascites
CCLE
54
ONCO-DG-1a
Ovarian adenocarcinoma
DSMZ
55
OV-7
Ovarian adenocarcinoma derived from solid tumour
ECACC
56
OV17R
Ovarian cancer ascites
ECACC
57
OV56
Ovarian cancer ascites
ECACC
58
OV-58
Ovarian cancer ascites
ECACC
59
OV-90
Ovarian cancer ascites
ATCC
60
OV-1063a
 
 
61
OVC1-PI 32
Ovary
NCBI
62
OVCAR-3
Ovarian cancer ascites
ATCC/NCBI
63
OVCAR-4
Ovarian adenocarcinoma
CCLE
64
OVCAR-8
Ovarian adenocarcinoma
CCLE
65
OVISE
Metastatic ovarian adenocarcinoma
JCRB/CCLE
66
OVK18
Ovarian adenocarcinoma
CCLE
67
OVKATE
Ovarian adenocarcinoma
JCRB
68
OVMANA
Ovarian adenocarcinoma
JCRB
69
OVMIUa
Ovarian adenocarcinoma
JCRB
70
OVMIU-IIa
Ovarian adenocarcinoma
JCRB
71
OVSAHO
Ovarian adenocarcinoma
JCRB
72
OVSAYOa
Ovarian adenocarcinoma
JCRB
73
OVTOKO
Ovarian adenocarcinoma
JCRB
74
PA-1
Ovarian cancer ascites
ATCC/JCRB/ECACC
75
PA-1/6TG-r
Ovarian cancer ascites
JCRB
76
PEA1
Ovarian cancer pleural effusion
ECACC
77
PEA2
Ovarian cancer ascites
ECACC
78
PEO1
Ovarian cancer ascites
ECACC
79
PEO4
Ovarian cancer pleural effusion
ECACC
80
PEO6
Ovarian cancer ascites
ECACC
81
PEO14b
Ovarian cancer ascites
ECACC
82
PEO16
Ovarian cancer ascites
ECACC
83
PEO23b
Ovarian cancer ascites
ECACC
84
RKN
Ovarian adenocarcinoma
JCRB
85
RMG-Ia
Ovarian adenocarcinoma
JCRB
86
RMG-II
Ovarian adenocarcinoma
JCRB
87
RMUG-La
Ovarian adenocarcinoma
JCRB
88
RMUG-S
Ovarian adenocarcinoma
JCRB
89
RTSGc
Ovarian adenocarcinoma
JCRB
90
SCC60
 
 
91
SK-OV-3
Ovarian cancer ascites
ATCC/NCBI/ECACC
92
SNU-8
Ovarian adenocarcinoma
CCLE
93
SNU-119
Ovarian adenocarcinoma
CCLE
94
SNU-840
Ovarian adenocarcinoma
CCLE
95
SW 626
Ovarian metastatic mass from colon tumour
ATCC/ECACC
96
TE 84.T
Ovarian adenocarcinoma
ATCC
97
TO14b
Metastatic omental mass from ovarian tumour
ECACC
98
TOV-21G
Malignant ovarian mass
ATCC
99
TOV-81D
Malignant ovarian mass
 
100
TOV-112D
Malignant ovarian mass
ATCC
101
TYK-nu
Ovarian adenocarcinoma
JCRB
102
TYK-nu.CP-r
Ovarian adenocarcinoma
JCRB
103
UC1-101
Ovarian adenocarcinoma
 
104 UC1-107    

aPossible cross contamination or misidentification (JCRB, DSMZ: Database of Cross-Contaminated or misidentified cell lines, Capes-Davis, A. and Freshney, R.I. Version 6.7, Table  1 27.6.2011). Cross contaminated with OVCAR-3 (ONCO-DG-1); bAll these cell lines were derived from the same patient.

Table 3.

Non-human cell line originated from the ovary

Cricetulus griseus – Chinese hamster
105
A2
Ovary
ECACC
106
A2H
Ovary; A2
ECACC
107
AR-EcoScreen
Ovary
JCRB
108
CHO
Ovary
ECACC/NCBI
109
CHO 1–15 500
Ovary
NCBI
110
CHO CD28
Ovary
NCBI
111
CHO-CHRM1
Ovary; CHO-K1
ECACC
112
CHO-CHRM2
Ovary; CHO-K1
ECACC
113
CHO-CHRM5
Ovary; CHO-K1
ECACC
114
CHO DG-44
Ovary
NCBI
115
CHO/dhFr-
Ovary
ECACC/DSMZ/NCBI
116
CHO/dhFr- Ac-free
Ovary; CHO/dhFr-
ECACC
117
CHO-FFAR2
Ovary; CHO-K1
ECACC
118
CHO-GPR120
Ovary; CHO-K1
ECACC
119
CHO/HGPRT
Ovary
JCRB
120
CHO (His9)
Ovary
JCRB
121
CHO-K1
Ovary; CHO
ECACC/JCRB/DSMZ
122
CHO-K1/SF
Ovary; CHO-K1
ECACC
123
CHO-OPRL1
Ovary; CHO-K1
ECACC
124
CHO (pMAM-HSluc)
Ovary
JCRB
125
CHO (pMAM-luc)
Ovary
JCRB
126
CHO Protein-Free
Ovary; CHO
ECACC
127
CHO-SSTR1
Ovary; CHO-K1
ECACC
128
GRL101 (KC7)
Ovary
ECACC
129
GRL101 (MIX)
Ovary
ECACC
130
M1WT3
Ovary; CHO-K1
ECACC
131
NCTC 4206
Peritoneum; B14FAF28-G3
ECACC
132
P22
Ovary
ECACC
133
RR-CHOKI
Ovary; CHO-K1
ECACC
134
T02J-7/10 (CHO-M3 (CHRM3))
Ovary; CHO-K1
ECACC
135
T02J-9/10 (CHO-H2 (HRH2))
Ovary; CHO-K1
ECACC
136
T02J-10/10 (CHO-GCGR (GCGR))
Ovary; CHO-K1
ECACC
137
T26J-1/09 (CHO-Beta-2 (ADRB2))
Ovary; CHO-K1
ECACC
138
T35J-5/09 (CHO-FFAR3 (FFAR3))
Ovary; CHO-K1
ECACC
139
UT-1
Ovary; CHO-K1
ECACC
140
XrS6
Ovary; CHO-K1
ECACC
141
Xrs6-hamKu80
Ovary; CHO-K1
ECACC
Mus musculus – mouse
142
OV3121
Ovary
JCRB
143
OV3121-ras4
Ovary
JCRB
144
OV3121-ras7
Ovary
JCRB
145
p53-def-MOSE
Ovary
JCRB
146
T-Ag-MOSE
Ovary
JCRB
Sus domesticus – Pig
147
AVG-16
Ovary follicle
ECACC
Spodoptera frugiperda – fall army worm
148
Sf 9
Pupal ovary
NCBI/ECACC
149
Sf 9 TitreHigh AC free
Pupal ovary; Sf 9 CL
ECACC
150
Sf 21
Pupal ovary
NCBI/ECACC
151
Sf 21 TitreHigh AC free
Pupal ovary; Sf 21 CL
ECACC
Esox lucius – Northern pike fish
152
PG
Ovary
ECACC
Ictalurus punctatus – channel catfish
153 CCO Ovary ECACC

It is noteworthy that cell line banks do not stock human cell lines described originating from primary tubal or peritoneal origin. However, only recently the isolation and culturing of normal ovarian and fallopian tube epithelial cells from the same healthy female has been described [35]. This finding may fill the current gap of knowledge and may help clarifying the apparent ambiguity of the origin of ‘ovarian cancer’ and enabling a clear distinction among ovarian, tubal, and peritoneal cancer at their later stages. However, peritoneal cell lines are still not available as are a subset of histologically distinct ovarian cancer cell lines such as borderline cancers, cystadenomas and carcinosarcomas.

The re-naming of cell lines causes constant confusion as respective annotations are often not found in cell banks. For example, 41 M cells are the same as OAW28 cells. Some cell lines have similar names and require caution in the selection of the cell line of choice: a majority of the animal cell lines and several human cell lines are derived from a parental line (e.g. A2780, CHO) and have been modified in vitro to display chemo resistance (e.g. cisplatin-resistant A2780CP) or different cellular factors. In addition, the verification of information given by the cell bank is difficult, because not all cell lines are linked to their original publications and their depositors are rarely mentioned.

One apparent shortcoming is that the ethnicity of the ovarian cancer patient from whom the tumour is derived is indicated in only 30.5%. Apart from the JCRB cell bank where all the deposited cell lines were derived from Japanese females (48.3%), the majority of samples where ethnical details are provided were from Caucasian females.

Since we know that different ethnic groups can have a propensity for specific genetic mutations, for example in the BRCA and APC genes of Ashkenazi Jews [36,37], it is extremely important to have cell lines that represent the spectrum of ethnic groups around the world. This will reduce the risk of an ethnic bias and ensure that research into different ethnic groups will allow the most benefit for these patients.

The role of genetic changes in the characterization of ovarian cancer cell lines

The (molecular) characterization of EOC in the clinics significantly depends on the presence and type of genetic alterations in the cancer and may define the treatment options and the patients’ outcome. The tumor origin where the cell lines derived from was not precisely provided in 51.2% (Table  4). Considering the clinico-pathological (histotype, FIGO stage, grade) as essential criteria to categorize EOC in type I and II tumours, the respective information provided by cell banks is not sufficient. The data review on available human ovarian cancer cell lines (n = 95) reflects that cell banks provide the histological subtype in 76.8% with discrepancies to original publications (Table  5), stage in 34.7%, and the initial grade in only 20%. In contrast, the information on chemotherapy resistance is provided adequately. Epithelial (-like) cells are characterized with epithelial or stromal markers in more than half (57.9%) of all cell lines, and out of these 85.4% had at least epithelial-like features. Another essential criterion is the doubling time that is provided in only 29.5%.

Table 4.

Origin of human ovarian cancer cell lines

 
 
Origin specified (cell line banks)
    Ascites Metastasis Ovary Pleural effusion
Origin specified (original references)
Ascites
9
0
5
0
Metastasis
0
2
6
0
Not specified
0
0
11
0
Ovary
0
0
9
0
  Pleural effusion 0 0 0 1

Table 5.

Histotypes of human ovarian cancer cell lines

 
 
Origin specified (cell line banks)
    Clear cell Endometrioid Mixed Mucinous Other Serous Unknown
Origin specified (original references)
Clear cell
6
0
0
0
0
0
0
Endometrioid
0
2
0
0
0
0
0
Mixed
0
0
1
0
0
0
1
Mucinous
0
0
0
3
2
0
0
Other
0
0
0
0
3
0
0
Serous
0
0
0
1
6
7
1
  Unknown 0 0 0 0 7 0 1

We also collected and evaluated data provided by cell banks in regards to molecular markers. This information was very limited and only few cell lines were evaluated for expression of progesterone (7.4%) and oestrogen (6.3%) receptors, vimentin (5.3%), TP53 mutations (4.2%), Her2/neu (3.2%), EpCAM (3.2%), and cytokines 7, 8, 17, 18, and 19 (ranging from 5.3% to 8.4%).

Potential risks of the use of cell lines for in vitro research

The misidentification and cross-contamination of cell lines is problematic in research and may increase the risk for false results and misinterpretations. The extent of misidentification is documented in a recent study wherein a panel of ovarian and endometrial cell lines was analysed by DNA profiling [38]. The authors found that 8 out of the 51 ovarian cancer cell lines were in fact breast cancer, teratocarcinoma, or cervical cancer cell lines and that2 normal endometrial cancer cells were in fact HeLa cervical cancer or MCF-7 breast cancer cells. Likewise, cross-contamination of cell lines, i.e. the accidental generation of mixed cell cultures, is not a lesser problem. Jäger et al. 2013 reported that the popular and frequently used KU7 urothelial carcinoma cell line was cross-contaminated years ago with HeLa cells [39]. Cross-contaminations may occur when multiple cell lines are cultured simultaneously (a practice that should be avoided) and becomes only apparent if multiple morphologies are suddenly observed but fatally remains unnoticed if cells have indistinguishable morphology.

Bacterial/fungal/yeast/mycoplasma contamination presents another problem adversely affecting research results. Of these, mycoplasma species are most likely to be detrimental to cell functioning. Unlike most bacterial, fungal or yeast infections, mycoplasma are macroscopically and microscopically undetectable; it may remain in culture for extended periods of time affecting cell growth, gene expression and overall cell functioning [40]. This may be one reason for why different research groups report contradictory findings. For this reason, Cell Bank Australia has collated a database of known cross-contaminated or misidentified cell lines based on the literature. Other cell banks such as the JCRB have also made an effort to screen the database and identified which of their own cell lines were originally misidentified (Table  1).

The unavailability of a considerable number of in vitro cell line models to the research community is also an issue. The problem is two-fold: firstly, there is no quality control of cells generated in individual laboratories when they are not deposited in a professional cell bank. Even when these cells are meticulously generated and cultured, independent quality checks and verifications are not possible. This flaw is overcome by directly contacting the laboratory where the cell lines were generated. This, however, can lead to the second problem; the passing on of cell lines from laboratory to the other, thereby bypassing the critical quality control cell banks. In the past it has been common practice to obtain cells from collaborating groups, and with the required permission, to again distribute these to other laboratories. Whilst this practice is in the spirit of research collaborations, it increases the risk of receiving contaminated or misidentified cell lines that, in turn, can be detrimental to research.

Conclusions

To ensure a unique quality of cancer research around the world we recommend that all cell lines used for research should be deposited in a cell bank and be readily accessible for all researchers. Ovarian cancer cell bank operators should provide development protocols and comprehensive clinical data for all commercially available cell lines. Depositors of cell lines should ensure that they have carefully collected all relevant clinical information from the donor individuals. This information includes: the exact origin of the cells, the stage during disease progression the cells were taken, the type of therapy the patient underwent prior to sample collection, the data on the patient’s survival, the ethnicity and family history (including known genetic alterations), and the preoperative plasma CA125 levels currently provided by only 5.3% of all human ovarian cancer cell lines. Additionally, we recommend that all cell bank operators conform to the same style of reporting the cell line information and only bank cells where all necessary information is available. This will ensure that the highest standard of research is maintained worldwide. Short tandem repeat (STR) profiling, a highly-sensitive method to detect cellular cross-contamination, should be performed by researchers for all newly generated cell lines and should be confirmed by the cell bank once deposited and prior to the sale of the cells. The service for STR profiling is provided by various laboratories, e.g. American Type Cell culture Collection (ATCC-USA, http://www.atcc.org), China Center for Type Culture Collection (CCTCC, http://www.cctcc.org), Australian Cell Bank ( http://www.cellbankaustralia.com), European Culture Collection of Cell Cultures (ECACC, http://www.hpacultures.org.uk), or German Cell Culture Collection (DSMZ, http://www.dsmz.de). From a recent study that histotyped standard ovarian cancer cell lines by short tandem repeats, immunohistochemistry, and mutation analysis it was concluded that the knowledge of the mutation status of cancer genes such as ARID1A and TP53 and of the general immunoprofile would be beneficial for the determination of the histotype of ovarian cancer cells [41]. Following the model of the Cancer Cell Line Encyclopedia (CCLE), we suggest the establishment of a centralized cell line database that would harbour all the relevant details of new cell lines and would be updated with new details in real time as experimental results are reported in the literature. This is believed to reduce the overlap of research performed and to continually improve the quality and appropriateness of future cell line studies. A cell bank professional with expertise in cancer research would be beneficial for researchers who need advice in correctly choosing the cell line appropriate for a specific research question. The expansion of the current offer of cell lines deposited in the cell banks by additional types of cells is desirable. These include primary, recurrent and metastatic ovarian-, tubal- and peritoneal cancers, a set of cell lines representing all known EOC histotypes, age-matched normal control OSE and tubal cells, and cell lines derived from primary, recurrent and metastatic tumours from the same patients at different progression time points. It is clear that worldwide collaborative efforts are to be taken to reach these recommendations, but we believe that this will be of benefit for the research results in the future.

Competing interests

The authors declare that they have no competing interests.

Authors’ contributions

FJ carried out literature research, data analysis and drafted the manuscript. SN carried out literature research drafted the manuscript. NFH drafted the manuscript. VAS conceived the review and drafted the manuscript. All authors read and approved the final manuscript.

Contributor Information

Francis Jacob, Email: francis.jacob@unibas.ch.

Sheri Nixdorf, Email: s.nixdorf@unsw.edu.au.

Neville F Hacker, Email: n.hacker@unsw.edu.au.

Viola A Heinzelmann-Schwarz, Email: viola.heinzelmann@usb.ch.

References

  1. Auersperg N, Wong AS, Choi KC, Kang SK, Leung PC. Ovarian surface epithelium: biology, endocrinology, and pathology. Endocr Rev. 2001;22:255–288. doi: 10.1210/edrv.22.2.0422. [DOI] [PubMed] [Google Scholar]
  2. Vaughan S, Coward JI, Bast RC Jr, Berchuck A, Berek JS, Brenton JD, Coukos G, Crum CC, Drapkin R, Etemadmoghadam D, Friedlander M, Gabra H, Kaye SB, Lord CJ, Lengyel E, Levine DA, McNeish IA, Menon U, Mills GB, Nephew KP, Oza AM, Sood AK, Stronach EA, Walczak H, Bowtell DD, Balkwill FR. Rethinking ovarian cancer: recommendations for improving outcomes. Nat Rev Cancer. 2011;11:719–725. doi: 10.1038/nrc3144. [DOI] [PMC free article] [PubMed] [Google Scholar]
  3. Siegel R, Naishadham D, Jemal A. Cancer statistics, 2013. CA Cancer J Clin. 2013;63:11–30. doi: 10.3322/caac.21166. [DOI] [PubMed] [Google Scholar]
  4. Jacob F, Goldstein DR, Fink D, Heinzelmann-Schwarz V. Proteogenomic studies in epithelial ovarian cancer: established knowledge and future needs. Biomarkers Med. 2009;3:743–756. doi: 10.2217/bmm.09.48. [DOI] [PubMed] [Google Scholar]
  5. Cho KR. Ovarian cancer update: lessons from morphology, molecules, and mice. Arch Pathol Lab Med. 2009;133:1775–1781. doi: 10.5858/133.11.1775. [DOI] [PMC free article] [PubMed] [Google Scholar]
  6. Landen CN Jr, Birrer MJ, Sood AK. Early events in the pathogenesis of epithelial ovarian cancer. J Clin Oncol. 2008;26:995–1005. doi: 10.1200/JCO.2006.07.9970. [DOI] [PubMed] [Google Scholar]
  7. Shih Ie M, Kurman RJ. Ovarian tumorigenesis: a proposed model based on morphological and molecular genetic analysis. Am J Pathol. 2004;164:1511–1518. doi: 10.1016/S0002-9440(10)63708-X. [DOI] [PMC free article] [PubMed] [Google Scholar]
  8. Kurman RJ, Shih Ie M. The origin and pathogenesis of epithelial ovarian cancer: a proposed unifying theory. Am J Surg Pathol. 2010;34:433–443. doi: 10.1097/PAS.0b013e3181cf3d79. [DOI] [PMC free article] [PubMed] [Google Scholar]
  9. Bast RC Jr, Hennessy B, Mills GB. The biology of ovarian cancer: new opportunities for translation. Nat Rev Cancer. 2009;9:415–428. doi: 10.1038/nrc2644. [DOI] [PMC free article] [PubMed] [Google Scholar]
  10. Jones S, Wang TL, Shih Ie M, Mao TL, Nakayama K, Roden R, Glas R, Slamon D, Diaz LA Jr, Vogelstein B, Kinzler KW, Velculescu VE, Papadopoulos N. Frequent mutations of chromatin remodeling gene ARID1A in ovarian clear cell carcinoma. Science. 2010;330:228–231. doi: 10.1126/science.1196333. [DOI] [PMC free article] [PubMed] [Google Scholar]
  11. Samartzis EP, Noske A, Dedes KJ, Fink D, Imesch P. ARID1A mutations and PI3K/AKT pathway alterations in endometriosis and endometriosis-associated ovarian carcinomas. Int J Mol Sci. 2013;14:18824–18849. doi: 10.3390/ijms140918824. [DOI] [PMC free article] [PubMed] [Google Scholar]
  12. Wiegand KC, Shah SP, Al-Agha OM, Zhao Y, Tse K, Zeng T, Senz J, McConechy MK, Anglesio MS, Kalloger SE, Yang W, Heravi-Moussavi A, Giuliany R, Chow C, Fee J, Zayed A, Prentice L, Melnyk N, Turashvili G, Delaney AD, Madore J, Yip S, McPherson AW, Ha G, Bell L, Fereday S, Tam A, Galletta L, Tonin PN, Provencher D. et al. ARID1A mutations in endometriosis-associated ovarian carcinomas. N Engl J Med. 2010;363:1532–1543. doi: 10.1056/NEJMoa1008433. [DOI] [PMC free article] [PubMed] [Google Scholar]
  13. Cancer Genome Atlas Research N. Integrated genomic analyses of ovarian carcinoma. Nature. 2011;474:609–615. doi: 10.1038/nature10166. [DOI] [PMC free article] [PubMed] [Google Scholar]
  14. Flesken-Nikitin A, Hwang CI, Cheng CY, Michurina TV, Enikolopov G, Nikitin AY. Ovarian surface epithelium at the junction area contains a cancer-prone stem cell niche. Nature. 2013;495:241–245. doi: 10.1038/nature11979. [DOI] [PMC free article] [PubMed] [Google Scholar]
  15. Dubeau L. The cell of origin of ovarian epithelial tumors and the ovarian surface epithelium dogma: does the emperor have no clothes? Gynecol Oncol. 1999;72:437–442. doi: 10.1006/gyno.1998.5275. [DOI] [PubMed] [Google Scholar]
  16. Dubeau L. The cell of origin of ovarian epithelial tumours. Lancet Oncol. 2008;9:1191–1197. doi: 10.1016/S1470-2045(08)70308-5. [DOI] [PMC free article] [PubMed] [Google Scholar]
  17. Costa MJ, Vogelsan J, Young LJ. p53 gene mutation in female genital tract carcinosarcomas (malignant mixed mullerian tumors): a clinicopathologic study of 74 cases. Mod Pathol. 1994;7:619–627. [PubMed] [Google Scholar]
  18. Runnebaum IB, Tong XW, Mobus VJ, Kieback DG, Rosenthal HE, Kreienberg R. p53 mutant His175 identified in a newly established fallopian tube carcinoma cell line secreting interleukin 6. FEBS Lett. 1994;353:29–32. doi: 10.1016/0014-5793(94)00953-8. [DOI] [PubMed] [Google Scholar]
  19. Crum CP. Intercepting pelvic cancer in the distal fallopian tube: theories and realities. Mol Oncol. 2009;3:165–170. doi: 10.1016/j.molonc.2009.01.004. [DOI] [PMC free article] [PubMed] [Google Scholar]
  20. Crum CP, Drapkin R, Miron A, Ince TA, Muto M, Kindelberger DW, Lee Y. The distal fallopian tube: a new model for pelvic serous carcinogenesis. Curr Opin Obstet Gynecol. 2007;19:3–9. doi: 10.1097/GCO.0b013e328011a21f. [DOI] [PubMed] [Google Scholar]
  21. Lee Y, Miron A, Drapkin R, Nucci MR, Medeiros F, Saleemuddin A, Garber J, Birch C, Mou H, Gordon RW, Cramer DW, McKeon FD, Crum CP. A candidate precursor to serous carcinoma that originates in the distal fallopian tube. J Pathol. 2007;211:26–35. doi: 10.1002/path.2091. [DOI] [PubMed] [Google Scholar]
  22. Crum CP, Drapkin R, Kindelberger D, Medeiros F, Miron A, Lee Y. Lessons from BRCA: the tubal fimbria emerges as an origin for pelvic serous cancer. Clin Med Res. 2007;5:35–44. doi: 10.3121/cmr.2007.702. [DOI] [PMC free article] [PubMed] [Google Scholar]
  23. Salvador S, Rempel A, Soslow RA, Gilks B, Huntsman D, Miller D. Chromosomal instability in fallopian tube precursor lesions of serous carcinoma and frequent monoclonality of synchronous ovarian and fallopian tube mucosal serous carcinoma. Gynecol Oncol. 2008;110:408–417. doi: 10.1016/j.ygyno.2008.05.010. [DOI] [PubMed] [Google Scholar]
  24. Chen EY, Mehra K, Mehrad M, Ning G, Miron A, Mutter GL, Monte N, Quade BJ, McKeon FD, Yassin Y, Xian W, Crum CP. Secretory cell outgrowth, PAX2 and serous carcinogenesis in the Fallopian tube. J Pathol. 2010;222:110–116. doi: 10.1002/path.2739. [DOI] [PMC free article] [PubMed] [Google Scholar]
  25. Chene G, Tchirkov A, Pierre-Eymard E, Dauplat J, Raoelfils I, Cayre A, Watkin E, Vago P, Penault-Llorca F. Early telomere shortening and genomic instability in tubo-ovarian preneoplastic lesions. Clin Cancer Res. 2013;19:2873–2882. doi: 10.1158/1078-0432.CCR-12-3947. [DOI] [PubMed] [Google Scholar]
  26. Jarboe E, Folkins A, Nucci MR, Kindelberger D, Drapkin R, Miron A, Lee Y, Crum CP. Serous carcinogenesis in the fallopian tube: a descriptive classification. Int J Gynecol Pathol. 2008;27:1–9. doi: 10.1097/pgp.0b013e31814b191f. [DOI] [PubMed] [Google Scholar]
  27. Kuhn E, Kurman RJ, Sehdev AS, Shih Ie M. Ki-67 labeling index as an adjunct in the diagnosis of serous tubal intraepithelial carcinoma. Int J Gynecol Pathol. 2012;31:416–422. doi: 10.1097/PGP.0b013e31824cbeb4. [DOI] [PMC free article] [PubMed] [Google Scholar]
  28. Auersperg N. Ovarian surface epithelium as a source of ovarian cancers: unwarranted speculation or evidence-based hypothesis? Gynecol Oncol. 2013;130:246–251. doi: 10.1016/j.ygyno.2013.03.021. [DOI] [PubMed] [Google Scholar]
  29. Perets R, Wyant GA, Muto KW, Bijron JG, Poole BB, Chin KT, Chen JY, Ohman AW, Stepule CD, Kwak S, Karst AM, Hirsch MS, Setlur SR, Crum CP, Dinulescu DM, Drapkin R. Transformation of the fallopian tube secretory epithelium leads to high-grade serous ovarian cancer in Brca;Tp53;Pten models. Cancer Cell. 2013;24:751–765. doi: 10.1016/j.ccr.2013.10.013. [DOI] [PMC free article] [PubMed] [Google Scholar]
  30. Seidman JD, Zhao P, Yemelyanova A. “Primary peritoneal” high-grade serous carcinoma is very likely metastatic from serous tubal intraepithelial carcinoma: assessing the new paradigm of ovarian and pelvic serous carcinogenesis and its implications for screening for ovarian cancer. Gynecol Oncol. 2011;120:470–473. doi: 10.1016/j.ygyno.2010.11.020. [DOI] [PubMed] [Google Scholar]
  31. Nik NN, Vang R, Shih Ie M, Kurman RJ. Origin and pathogenesis of pelvic (ovarian, tubal, and primary peritoneal) serous carcinoma. Annu Rev Pathol. 2014;9:27–45. doi: 10.1146/annurev-pathol-020712-163949. [DOI] [PubMed] [Google Scholar]
  32. Kuhn E, Kurman RJ, Vang R, Sehdev AS, Han G, Soslow R, Wang TL, Shih Ie M. TP53 mutations in serous tubal intraepithelial carcinoma and concurrent pelvic high-grade serous carcinoma–evidence supporting the clonal relationship of the two lesions. J Pathol. 2012;226:421–426. doi: 10.1002/path.3023. [DOI] [PMC free article] [PubMed] [Google Scholar]
  33. Goodman MT, Shvetsov YB. Incidence of ovarian, peritoneal, and fallopian tube carcinomas in the United States, 1995–2004. Cancer Epidemiol Biomarkers Prev. 2009;18:132–139. doi: 10.1158/1055-9965.EPI-08-0771. [DOI] [PMC free article] [PubMed] [Google Scholar]
  34. Domcke S, Sinha R, Levine DA, Sander C, Schultz N. Evaluating cell lines as tumour models by comparison of genomic profiles. Nat Commun. 2013;4:2126. doi: 10.1038/ncomms3126. [DOI] [PMC free article] [PubMed] [Google Scholar]
  35. Merritt MA, Bentink S, Schwede M, Iwanicki MP, Quackenbush J, Woo T, Agoston ES, Reinhardt F, Crum CP, Berkowitz RS, Mok SC, Witt AE, Jones MA, Wang B, Ince TA. Gene Expression Signature of Normal Cell-of-Origin Predicts Ovarian Tumor Outcomes. PLoS One. 2013;8:e80314. doi: 10.1371/journal.pone.0080314. [DOI] [PMC free article] [PubMed] [Google Scholar]
  36. Im KM, Kirchhoff T, Wang X, Green T, Chow CY, Vijai J, Korn J, Gaudet MM, Fredericksen Z, Shane Pankratz V, Guiducci C, Crenshaw A, McGuffog L, Kartsonaki C, Morrison J, Healey S, Sinilnikova OM, Mai PL, Greene MH, Piedmonte M, Rubinstein WS, Hebon, Hogervorst FB, Rookus MA, Collee JM, Hoogerbrugge N, van Asperen CJ, Meijers-Heijboer HE, Van Roozendaal CE, Caldes T. et al. Haplotype structure in Ashkenazi Jewish BRCA1 and BRCA2 mutation carriers. Hum Genet. 2011;130:685–699. doi: 10.1007/s00439-011-1003-z. [DOI] [PMC free article] [PubMed] [Google Scholar]
  37. Bahar AY, Taylor PJ, Andrews L, Proos A, Burnett L, Tucker K, Friedlander M, Buckley MF. The frequency of founder mutations in the BRCA1, BRCA2, and APC genes in Australian Ashkenazi Jews: implications for the generality of U.S. population data. Cancer. 2001;92:440–445. doi: 10.1002/1097-0142(20010715)92:2<440::AID-CNCR1340>3.0.CO;2-O. [DOI] [PubMed] [Google Scholar]
  38. Korch C, Spillman MA, Jackson TA, Jacobsen BM, Murphy SK, Lessey BA, Jordan VC, Bradford AP. DNA profiling analysis of endometrial and ovarian cell lines reveals misidentification, redundancy and contamination. Gynecol Oncol. 2012;127:241–248. doi: 10.1016/j.ygyno.2012.06.017. [DOI] [PMC free article] [PubMed] [Google Scholar]
  39. Jager W, Horiguchi Y, Shah J, Hayashi T, Awrey S, Gust KM, Hadaschik BA, Matsui Y, Anderson S, Bell RH, Ettinger S, So AI, Gleave ME, Lee IL, Dinney CP, Tachibana M, McConkey DJ, Black PC. Hiding in plain view: genetic profiling reveals decades old cross contamination of bladder cancer cell line KU7 with HeLa. J Urol. 2013;190:1404–1409. doi: 10.1016/j.juro.2013.03.009. [DOI] [PMC free article] [PubMed] [Google Scholar]
  40. Zhang S, Wear DJ, Lo S. Mycoplasmal infections alter gene expression in cultured human prostatic and cervical epithelial cells. FEMS Immunol Med Microbiol. 2000;27:43–50. doi: 10.1111/j.1574-695X.2000.tb01410.x. [DOI] [PubMed] [Google Scholar]
  41. Anglesio MS, Wiegand KC, Melnyk N, Chow C, Salamanca C, Prentice LM, Senz J, Yang W, Spillman MA, Cochrane DR, Shumansky K, Shah SP, Kalloger SE, Huntsman DG. Type-specific cell line models for type-specific ovarian cancer research. PLoS One. 2013;8:e72162. doi: 10.1371/journal.pone.0072162. [DOI] [PMC free article] [PubMed] [Google Scholar]

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