The precise aetiology of the majority of breast cancers is elusive, which contrasts with the estimated 5–10% that are caused by inherited mutations. It is clear that breast cancer presents as a collection of distinct disease types that differ in disease progression, treatment response and disease-free survival. In addition to conventional pathology, emerging technologies, including micro-arrays, have proven to be excellent tools in enhancing our understanding of individual breast cancers and providing assistance in treatment decision making in clinically relevant subgroups 1. Initial observations, indeed most of our current understanding of chromosome abnormalities came from conventional cytogenetics. The importance of DNA copy number alterations has been demonstrated in many tumours 2. More recently, the results of array comparative genomic hybridization (array-CGH) analysis of tumour tissues have been described from several perspectives, including identification of subgroups (class discovery); identification of genes that are involved in tumour progression, metastasis and treatment response; identification of candidate oncogenes (in genetic amplifications) or tumour suppressors (in homozygous deletions); and classification of hereditary cancers. A few studies have also described CGH-based distinctions between sporadic and familial cases of breast cancer. Among familial cases, further classification into BRCA1, BRCA2, or 'other genetic risk factor(s)' is useful in these families in general but also for potential additional gene discovery.

Array-CGH technology is a fairly recent and important upgrade to the groundbreaking (conventional, metaphase chromosome) CGH technology 34, and it is applied to detect chromosomal DNA copy number alterations (CNA) in cells or tissues that occur as a result of genomic instability. CGH technology caused a paradigm shift in (clinical) cytogenetics because it avoids the need to culture (tumour) cells. This is perhaps the main reason why there was considerable over-representation of information on nonsolid tumours in cytogenetic databases. Array-CGH can measure genome-wide copy numbers in an unprecedented and objective manner. More importantly, complex karyotypes – a hallmark of many tumours – could be analyzed, including those too complex for G-banding because CGH readout is done on normal metaphase chromosomes. Last but not least, CGH was spectacular step forward because it preceded and did not require the completion of the human genome (draft) sequence 5. It was not until 1998, with knowledge of the human sequence, that array-CGH began to replace conventional CGH 6, again with some major improvements.

Array-CGH is superbly reviewed elsewhere 789101112, including its development, initial challenges and ultimate benefits relative to conventional CGH. However, application of array-CGH to breast cancer research has not specifically been addressed. In this review, we discuss some of the prospects of using array-CGH data to elucidate the process of carcinogenesis in breast cells and its possible impact on diagnostic stratification for clinical management. The review addresses the two goals of array-CGH in breast cancer, which can be summarized as follows: (novel) gene discovery in relation to subtypes, stage, or prognosis of breast cancer; and building class discovery tools for classification of independent breast cancers, regardless of the primary aim of identifying genes.

The effective resolution, sensitivity and reproducibility of array-CGH are constantly being enhanced. Although the maximal technical resolution of CGH is now approximately 140 kb 13, the resolution of the majority of published array-CGH studies is in the order of 1 or 2 Mb. This is the average spacing of probes along the genome but varies considerably by region. The sensitivity of nearly all platforms is sufficient to detect one-copy gains and losses, provided that at least 70% of the cells in the sample are tumour cells. Thus, the detection limits decrease with a combination of the following parameters; smaller aberration size (in bases), smaller aberration amplitude (copy number) and smaller tumour subclone representation.

Study of gene expression using array technology has garnered enormous popularity, and continues to generate high-impact classifiers of tumour type and disease progression 3424344. One must keep in mind that expression arrays and array-CGH measure different things, which are not always easily correlated. Expression arrays measure relative abundance of specific mRNA transcripts and CGH measures relative copy numbers of genomic DNA regions in a sample. The expression levels per gene vary enormously even in normal cells, depending, for instance, on cell type and cell cycle. The chromosomal fragment (or gene) copy numbers as measured by array-CGH show much less variation, being one or two copies in normal cells, and perhaps ranging between none and 20 copies in tumour cells. It is therefore difficult to correlate expression data with genomic data directly.

Several studies that have correlated DNA copy number data (CGH) with expression profiles have been published 374546. They indicate a significant correlation between copy number and gene expression. In regions of high-level amplification, 44–62% of genes were reported to be over-expressed 4546, compared with just 12% of all genes. The relation may in some cases be less straightforward, probably due to the complexity of gene regulation, including pathway feedback loops. An illustration for this is that breast cancers with ERBB2 (17q21) amplification almost invariably overexpress the gene, which contrasts with only 55% of cases with a gain of ERBB1 (7p12) 47. Arrays that support measurement of DNA as well as RNA include cDNA, oligo-, and single nucleotide polymorphism (SNP) arrays. The benefits of dual use are limited because CGH signals become critically low on short probes; short-probe (high-complexity) arrays tend to be much more expensive then BAC arrays; and the reference sample in expression profiling is not defined but at best held constant across a series of experiments, as opposed to using a completely 2n (normal karyotype) reference for array-CGH.

Another important advantage of CGH compared with expression arrays is that CGH can be conducted reliably using archival formalin-fixed paraffin-embedded material 26484950. Although there is evidence that archival material is also suited to expression analysis, it is only with recently fixed tissues and only with much effort 51.

One major application of CGH is in the analysis of cancer genomes for genome-wide copy number changes. The resolution of classic chromosomal CGH is limited by the highly condensed state of metaphase chromosomes and further by the optical resolution of the microscopes used to capture the hybridization signals. In addition, chromosome condensation may vary from metaphase spread to metaphase spread. The analysis software normalizes all chromosomes and assumes linear condensation of all chromosomes. As a result, the precise location of aberrations becomes uncertain, which reduces the true effective resolution. In contrast, the resolution of array-CGH is limited only by the density and average length of the probe set printed on the array. Compared with metaphase-CGH, one problem – especially with earlier versions of array-CGH – was the uncertainty regarding the genomic location of the clones, which is dependent on the version of the 'genome build' of the human genome. The ability to detect a change of one copy for both technologies is roughly similar but highly influenced by the frequent admixture of nontumour cells in the sample, as well as by heterogeneity of the tumour tissue (i.e. generally not all cells will have the same ploidy for all chromosomal regions). Both factors are important in the analysis of breast cancer, because breast tumours are heterogeneous and may contain significant proportions of normal cells. Therefore, as a rule CGH should be performed only on tissue samples containing 70% or more tumour cells, or one must meet this requirement through enrichment by macrodissection, (laser capture) micro-dissection, or flow sorting (fluorescence-activated cell sorting), followed by some means of DNA amplification 2752.

Contrary to mRNA content, which for a given gene in a cell can range between no copies (not expressed) up to many thousands, the chromosome content of normal (reference) cells is extremely stable (2n, or diploid); when it is unstable, as is frequent in cancer cells, it at least remains quite discrete. This means that extensive regions of the genome are usually still balanced as in the diploid (2n or unchanged) or tetraploid (duplicated) state. Unbalanced regions exist either as homozygous loss (0 copies), heterozygous loss (1 copy or loss of heterozygosity [LOH]), gain (~3 or 4 copies), and amplifications (~5 or more copies). The distinction between diploid and triploid or tetraploid genomes cannot be detected by array-CGH but is best determined by some independent cell-based method such as fluorescent in situ hybridization (FISH).

If we reverse the perspective, array-CGH data can also tell us something about tumours. This is similar to how cytogenetic data were used to define subgroups in breast cancer that correlated with histological type, grade and mitotic activity of the tumour 5354. CGH has been used to classify breast tumours 5556. Because breast cancer is a disease with high levels of chromosome instability, it can readily be studied by CGH. Results from various classification studies have indicated that many gains and losses show recurrences anywhere between 20% and 80% of all tumours in a class, depending on the region and the cancer subtype investigated. Some recurrences exhibit sufficient differential gains or losses between classes to permit their use for classification, as in the case of inherited BRCA1 and BRCA2 mutations 5556. Certain regions such as 1q and 8q almost exclusively exhibit gain and rarely loss, whereas 16q often shows loss but hardly ever gain.

Robust classification procedures require more than counting frequencies of specific aberrations in various tumour types. It is important to appreciate that even a significant correlation of, for instance, 16q loss, which is more frequent in lobular breast cancer 57, provides limited statistical prediction power for an individual prospective case. This requires more rigorous, iterative methods of feature and model selection, followed by cross-validations and external validations. Provided that the correct methods are used, we believe that array-CGH can be useful for identifying distinct breast tumour subtypes, and can help to define them further, similar to the study reported by Jonsson and coworkers 58.

Cancer is the result of a myriad of genetic and epigenetic alterations. Identification of the causal perturbations that confer malignant transformation is a central goal in cancer biology. CGH is a powerful tool for investigating tumours in a genome-wide manner for such candidate regions. This strategy was successfully used to identify c-Myc, Her2Neu, Rab25 and a range of other potential oncogenes 325960. Vice versa, beginning with knowledge of the causal gene for the tumour, CGH has been useful in elucidating the extent of specific as well as recurrent aberrations in tumours such as those associated with mutations in BRCA1, BRCA2, or P53 in both mouse 61 and human 5556586263. Genomic instability occurs is still not fully understood. Recently, a number of possible mechanisms focusing on the fidelity of chromosome segregation and/or DNA repair have been proposed 6465, which may hold some indirect clues as to how breast tumour CGH profiles in BRCA1 mutation carriers are different from those in sporadic cases, but they still fail to explain why. While progress is made to elucidate further the precise nature of genomic instability, the resulting specificity of CGH profiles has already been put to good use.

Any review of the analysis of chromosomal copy numbers in breast cancer by array-CGH would be incomplete without mention of some related technologies (e.g. genome-wide LOH analysis, SNP [haplotype] analysis, CESH 9499 [also called expressive genomic hybridization 100], large-scale PCR 101 and expression array studies) that often have similar or overlapping goals, including classification, clinical prognostication, defining treatment subgroups, finding novel genes, and so on.

Several studies have already demonstrated the feasibility of performing genome-wide LOH and SNP analysis, for example by using Illumina bead-array technology on formalin-fixed paraffin-embedded tumour tissues 102103104. These technologies have a clear advantage over (array) CGH in that they extract haplotype information in addition to chromosome copy number. This is especially relevant in chromosomal uniparental isodisomy, inherited or acquired through mitotic recombination resulting in variably extended stretches of homozygosity (i.e. LOH) in the absence of copy number changes. This has been observed in breast cancer and may be more frequent then is generally acknowledged 105.

Array-CGH is a reliable, sensitive and high-resolution method that is highly automated compared with metaphase-CGH, which it is now replacing; thus, array-CGH is expected to generate an enormous amount of data in the coming years. One limitation of all current breast cancer array-CGH studies is the limited number of samples used per study. It poses the classic risk for over-fitting for as long as the average study contains two orders of magnitude more features (i.e. probes) then samples. One way to tackle this limitation is to have available the combined data sets or a repository for meta-analyses of CGH data, histological data, immunostaining data, clinical data, and so forth.

This review has described the two separate goals of CGH in breast cancer: gene discovery and class discovery. For both we have given successful examples. An example of gene identification is TAFA1, the significance of which in cell transformation was found by array-CGH and was verified extensively with other methods 93. These data clearly prioritize this locus for further functional studies of this relatively uncharacterized gene. An example of class prediction by array-CGH is the study Jonsson and coworkers 58, who built classifiers for BRCA1 and BRCA2 breast tumours.

One further conclusion of our review of the array-CGH literature is that the known heterogeneity of breast cancer also seems reflected in array-CGH data, such that multiple types of profiles have been reported, sometimes with clear but sometimes with less clear associations with known types of breast cancer. The fact is that the number of described subtypes of breast cancer increases with increasing sensitivity and resolution of newer methods. Although novel technology has no a priori knowledge of the problem analyzed, one would generally be satisfied if a new technology would permit enhanced stratification of disease entities. However, in breast cancer we see a trend toward discovery of more subgroups that sometimes appear independent of more traditional classification features, such as grade, size and immunochemistry (e.g. P53, oestrogen receptor, progesterone receptor, ERBB2) 96. One interpretation is that the within group variability, for instance, among all grade III cases or all oestrogen receptor negative cases is still quite large. In our opinion, this could account for the independent clustering when using CGH data compared with other tumour characteristics, even when the same tumour set is studied.

In the near future, when increasing numbers of studies generate higher resolution data in conjunction with allele-specific information, such as produced by SNP arrays or Illumina bead arrays, it may become possible also to elucidate some effects of genetic backgrounds or genotypes on CGH as a proxy for genomic instability. Nevertheless, genetic background appears to impact on CGH profiles 106, and this type of information should hopefully teach us more about the biology of chromosomal instability. This touches on a possible relation between CGH profiles and human genetic diversity that can best be studied on genome-wide SNP/CGH arrays and could be extremely useful in locating putative (median and low risk) breast cancer genes.

Despite the current trend in which oligo array-CGH is gradually replacing BAC array-CGH because of its flexibility (clone-less, fast and custom print-on-demand, and probably the most powerful advantage of assessing copy number and allele information simultaneously), it seems that BAC arrays will remain important for profiling DNA from formalin-fixed material.

BAC = bacterial artificial chromosome; CESH = comparative expressed sequence hybridization; CGH = comparative genomic hybridization; CNA = copy number alterations; FISH = fluorescent in situ hybridization; LOH = loss of heterozygosity; PCR = polymerase chain reaction; SNP = single nucleotide polymorphism.

The authors declare that they have no competing interests.