Journal of Histochemistry and Cytochemistry, Vol. 51, 1343-1353, October 2003, Copyright © 2003, The Histochemical Society, Inc.


ARTICLE

Chromosomal Variations Within Aneuploid Cancer Lines

Takahiro Isaka1,2,a, Andrea L. Nestor1,a, Tadahiro Takada2,a, and David C. Allisona
a Departments of Surgery, Physiology and Molecular Medicine, and the MCO Microscopy Imaging Center, Medical College of Ohio, Toledo, Ohio

Correspondence to: David C. Allison, Medical College of Ohio, 3035 Arlington Ave., Toledo, OH 43614-5804. E-mail: dallison@mco.edu


  Summary
Top
Summary
Introduction
Materials and Methods
Results
Discussion
Literature Cited

Aneuploid cancers exhibit a wide spectrum of clinical aggressiveness, possibly because of varying chromosome compositions. To test this, karyotypes from the diploid CCD-34Lu fibroblast and the aneuploid A549 and SUIT-2 cancer lines underwent fluorescence in situ hybridization (FISH) and DAPI counterstaining. The number of DAPI-stained and FISH-identified chromosomes, 1-22, X,Y, as well as structural abnormalities, were counted and compared using the {chi}2, Mann–Whitney rank sum test and the Levene's equality of variance. Virtually all of the evaluable diploid CCD-34Lu karyotypes had 46 chromosomes with two normal-appearing homologues. The aneuploid chromosome numbers per karyotype were highly variable, averaging 62 and 72 for the A549 and SUIT-2 lines, respectively. However, the A549 chromosome numbers were more narrowly distributed than the SUIT-2 karyotype chromosome numbers. Furthermore, 25% of the A549 chromosomes had structural abnormalities compared to only 7% of the SUIT-2 chromosomes. The chromosomal compositions of the aneuploid A549 and SUIT-2 cancer lines are widely divergent, suggesting that diverse genetic alterations, rather than chance, may govern the chromosome makeups of aneuploid cancers. (J Histochem Cytochem 51:1343–1353, 2003)

Key Words: aneuploidy, karyotypes, chromosomal abnormalities, cell lines, fluorescence in situ, hybridization


  Introduction
Top
Summary
Introduction
Materials and Methods
Results
Discussion
Literature Cited

SOLID CANCERS can be classified by flow cytometric or image analysis DNA measurements as having diploid (2C) or aneuploid DNA contents (Swift 1950a , Swift 1950b ; Crissman and Tobey 1974 ; Bedi and Goldstein 1976 ; Allison et al. 1981 ; Hardie et al. 2002 ). Aneuploid chromosome compositions are felt to be due to largely random structural rearrangements and chromosome losses/gains from non-disjunctions and multipolar mitoses, most often originally occurring from tetraploid (4C) precursor cells (Boveri 1902 ,1964; Hsu and Moorhead 1956 ; Makino 1956 ; Shackney et al. 1989 ; Levine et al. 1991 ; Rasnick 2002 ). However, this mechanism of aneuploidy formation does not explain the wide spectrum of clinical aggressiveness of aneuploid human cancers (Anniko et al. 1984 ; Armitage et al. 1985 ; van den Ingh et al. 1985 ; Joensuu et al. 1986 , Joensuu et al. 1989 ; Hedley et al. 1987 ; Scott et al. 1987 ; Christiansen and Lampert 1988 ; Hamming et al. 1988 ; Joensuu and Klemi 1988 ; Jones et al. 1988 ; Kheir et al. 1988 ; Taylor et al. 1988 ; Clark et al. 1989 ; Ellis et al. 1989 ; Donohue et al. 1990 ; Heimann et al. 1990 ; Allison et al. 1991 , Allison et al. 1998 ; Eskelinen et al. 1991 ).

There has been a recent understanding of the DNA repair, cell cycle, and mitotic checkpoints (Nurse 1997 , Nurse 2000 ; Paulovich et al. 1997 ). It is possible that various derangements of these regulatory gene networks might cause differing aneuploid tumor chromosomal compositions and lead to various levels of genetic instability and clinical aggressiveness for these cancers. To test whether or not wide chromosomal variations might occur among different aneuploid cell populations, we have performed a fluorescence in situ hybridization (FISH) study of the karyotypic chromosomes of one diploid (CCD-34Lu, control) and two aneuploid (A549 and SUIT-2) cancer cell lines. The karyotypes of the diploid CCD-34Lu line almost invariably contained 46 chromosomes with two normal appearing copies of each FISH-localized homologue. However, the two aneuploid cancer lines showed wide differences in their mean karyotypic chromosome numbers, variations in the numbers of individual chromosomes per karyotype, and the occurrence of FISH-identified structural chromosome abnormalities.


  Materials and Methods
Top
Summary
Introduction
Materials and Methods
Results
Discussion
Literature Cited

Cell Culture
The diploid CCD-34Lu cell line (derived from female lung tissue) and the aneuploid A549 line (derived from a male lung carcinoma) were obtained from American Type Culture Collection (Rockville, MD). The SUIT-2 aneuploid cell line (derived from a male pancreatic adenocarcinoma) was a generous gift from Dr. Takeshi Iwamura (Department of Surgery, Miyazaki Medical College, Miyazaki, Japan). Each of the cell lines was grown as monolayers in DMEM (CCD-34Lu and A549) or McCoy's (SUIT-2) medium containing L-glutamine, 10% FBS (Invitrogen; Carlsbad, CA), and sodium bicarbonate (Amersham Life Sciences; Arlington Heights, IL) (Nestor et al. 2001 ). Cells were harvested from the tissue culture flasks in exponential growth phase, treated with "hypo," and dropped onto glass slides from 25 cm. The slides were not flamed but were allowed to air-dry and stored until hybridization.

FISH Chromosomal Localizations
This method has previously been described in detail (Allison and Nestor 1999 ). Centromere-specific probes, used when available, and chromosome "paints" were labeled with Spectrum Orange or Spectrum Green (Vysis; Downers Grove, IL). Slides were incubated in a 2 x SSC solution (pH 7.0) for 30 min, followed by dehydration. The centromeric/paint probe mixtures consisted of 1 µl Spectrum Orange and Spectrum Green probes, 1 µl ddH2O, and 7 µl hybridization solution (50% formamide/2 x SSC/10% dextran sulfate). The probe mixtures were denatured at 70C for 5 min and held at 4C until use. Cells hybridized to the probe mixtures were denatured for 2 (paint mixture) and 5 (centromeric mixture) min, in 70% formamide/2 x SSC solution at pH 7.0. This was followed by slide incubation overnight with probe solution in a humidified chamber at 43C, washing in 50–65% formamide/2 x SSC solution (pH 7.0), and counterstaining with DAPI. The Spectrum Orange fluorochromes were localized with a rhodamine-specific filter cube, BP510-560, FT580, LP590, with a Zeiss microscope under epifluorescence optics with a Neofluar x100 oil immersion lens (NA 1.30; Carl Zeiss, Thornwood, NY). The Spectrum Green fluorochromes were visualized with filter cube BP450–490, FT510, LP520, and a G365, FT395, LP420 filter cube was used for the DAPI stain. Analogue images were digitized and processed for removal of extraneous background fluorescence by Probevision software (Applied Imaging; Santa Clara, CA).

FISH Karyotypic Chromosome Distributions
The number of chromosomes localized with chromosome-specific FISH probes (1–22, X,Y) were counted in at least 20 separate karyotypes of each cell line. The numbers of each FISH-localized chromosome counted in separate karyotypes of the same line were placed in the columns of a rectangular matrix with 24 column headings for each chromosome 1, 2, ... 22, X, and Y. The sum of each row of this matrix gives a total number of chromosomes of one "pseudo-karyotype." Random changing of the positions of the chromosome numbers in each column, relative to its neighbors, allows the generation of "pseudo-karyotypic" chromosome distributions for each line. The mean chromosome numbers and standard deviations of such distributions stabilize at total karyotype number (n) values >100 (data not shown).

Statistical Analysis
Statistical software packages used for data analysis were version 2.03 of Sigma Stat and Version 10.1 of the SPSS for Windows program. Differences in the frequency of chromosome abnormalities were compared using the {chi}2 test in a 2 x 2 contingency table. Analysis of the difference in mean DAPI-stained and FISH-identified chromosome numbers of each cell line was performed using the Mann–Whitney rank sum test. The DAPI-stained and "FISH-pseudo" chromosome distribution spreads were analyzed by Levene's test of equality of variance. Finally, the correlation coefficient (r) was used to measure the strength of association between the mean number and variability of the individual DAPI-stained and FISH-identified chromosomes. Values of the correlation coefficient (r) ranging between 0 and 0.33 were not correlated, whereas values between 0.33 and 0.66 and between 0.66 and 1 were weakly and highly correlated, respectively.


  Results
Top
Summary
Introduction
Materials and Methods
Results
Discussion
Literature Cited

Karyotypes and FISH-identified Chromosomes
FISH was used to examine the individual chromosomes of three cell lines: A normal lung fibroblast cell line, CCD-34Lu, with a diploid complement of 46 chromosomes, was compared to the aneuploid A549 (lung carcinoma) and SUIT-2 (pancreatic adenocarcinoma) cell lines. Fig 1A–1C show CCD-34Lu, A549, and SUIT-2 karyotypes with 46, 65, and 81 DAPI-stained (blue) chromosomes, respectively. The CCD-34Lu karyotype in Fig 1A shows the expected diploid number of two FISH-localized centromeric probes for chromosomes 1 (red) and 16 (green). However, the A549 karyotype in Fig 1B, showing co-localization of two FISH "paint probes" identifying chromosomes 19 (red) and 1 (green), clearly reveals four copies of chromosome 19. Similarly, the SUIT-2 karyotype in Fig 1C, co-localized with FISH probes specific for the centromeres of chromosomes 17 (red) and 4 (green), shows six and four copies of these chromosomes, respectively. Therefore, the two aneuploid karyotypes (Fig 1B and Fig 1C) both show an elevation in the number of DAPI-stained chromosomes to well above the 46 diploid number (Fig 1A) and highly variable numbers of the FISH-identified homologues (Fig 1B and Fig 1C).



View larger version (47K):
[in this window]
[in a new window]
 
Figure 1. Localization of chromosome-specific FISH probes in DAPI-stained karyotypes. The diploid CCD-34Lu (A) and aneuploid A549 (B) and SUIT-2 (C) cell lines were hybridized with specific centromeric and paint DNA probes specific for chromosomes (1 red, 16 green), (19 red, 13 green), and (17 red, 4 green). (D) A composite karyotype of FISH-identified chromosomes of the diploid CCD-34Lu line. (E) FISH-localization of (Ea) extrachromosomal fragments (ECFs) found in the aneuploid SUIT-2 line showing two normal centromeric localizations of the FISH probes for chromosome 1 and in five ECFs from the same karyotype. (Eb) Normal chromosome 19 paint localization next to chromosome 19 breaks and refusions to another chromosome(s) found in the same karyotype of the aneuploid A549 line. (Ec) Centromeric localization of the FISH probe in a normal chromosome 2 and in several abnormally placed telomeric regions classified as ENDs in the same karyotype of the A549 line. (Ed) Fusions found in both aneuploid cell lines with centromeric chromosome probes labeled in red (r) and green (g) from left to right: 18r/16g, 7r/10g, 20r/9g, and 18r/10g.

FISH probes specific for all human chromosomes (1–22 X,Y) were hybridized to karyotypes of each of the three lines. The female CCD-34Lu karyotypes did not hybridize with FISH probes specific for the Y chromosome. Fig 1D shows a composite karyotype of the CCD-34Lu cell line showing localization of centromeric (1–4, 6–12, 15–18, 20, X) and paint (5, 13, 14, 19, 21, 22) FISH probes. Each of the CCD-34Lu chromosomes have normal morphology and appropriate FISH probe localizations (Fig 1D). Conversely, the aneuploid A549 and SUIT-2 lines often had FISH-identified chromosomes with structural abnormalities such as extrachromosomal fragments (ECFs), breaks, end localizations (ENDs), and fusions (Fig 1Ea–1Ed).

FISH Chromosome Numbers
We counted the numbers of FISH-localized homologues for each chromosome (1–22, X,Y) in at least 20 karyotypes of each cell line. All but six of the female CCD-34Lu karyotypes 332/338 showed two normal-appearing homologues of each somatic and sex (X) chromosome (Fig 1D). In the karyotypes lacking two homologues, the total number of DAPI-stained chromosomes was less than 46. Because no triploid or higher numbers of individual FISH-localized chromosomes were found in the CCD-34Lu karyotypes, it is likely that the CCD-34Lu karyotypes with less than 46 chromosomes were due to cytogenetic preparation error caused by some chromosomes washing off the slides.

The average copy number of FISH-identified A549 and SUIT-2 chromosomes per karyotype, plotted for each individual chromosome in Fig 2A and Fig 2B, usually varied from the diploid value of two found for the CCD-34Lu karyotypes (Fig 1A–1D). There was often wide variability of averages and ranges of copy numbers of the FISH-identified aneuploid chromosomes in different karyotypes of the same line, as evidenced by the wide standard deviation (SD) bars for many of the individual FISH-localized chromosome counts (Fig 2A and Fig 2B). However, the average chromosome copy number of a given individual. FISH-identified chromosome was often different in the A549 and SUIT-2 karyotypes. For example, in the A549 line there were 5.8 ± 1.40 copies of chromosome 1 per karyotype (Fig 2A), but the SUIT-2 karyotypes only averaged 4.0 ± 1.0 copies of chromosome 1 (Fig 2B). Fig 2C shows a plot of the mean copy numbers of the individual FISH-identified A549 chromosomes on the Y-axis vs the mean copy numbers for the same SUIT-2 chromosomes on the X-axis. Only a weak correlation (r=0.543) was found between the average chromosome copy numbers of the two lines. The copy number variation of individual, FISH-identified chromosomes also differed between the two aneuploid lines. Fig 2D shows the percent coefficients of variation (% CVs; SD divided by the mean multiplied by 100) of each individual FISH-identified A549 karyotypic chromosome count plotted on the Y-axis vs the % CVs of the counts of the same SUIT-2 chromosomes on the X-axis. Again, only a weak correlation (r=0.478) was found between the variability of individual A549 and SUIT-2 chromosome copy numbers (Fig 2D).



View larger version (23K):
[in this window]
[in a new window]
 
Figure 2. Average numbers of FISH-localized individual chromosomes in different karyotypes of the aneuploid A549 and SUIT-2 lines: mean number of chromosome-specific FISH probes ±SD for each individual chromosome in the A549 (A) and SUIT-2 (B) lines. (C) Correlation plot of the mean chromosome numbers and % CVs (D) of each FISH-identified individual chromosome of the A549 vs SUIT-2 line.

FISH-identified Chromosome Abnormalities
The numbers of FISH-identified structurally abnormal chromosomes differed significantly (p<0.001) among the karyotypes of the three lines (Table 1). No abnormalities were found in any of the FISH-identified CCD-34Lu chromosomes scanned (0/651; Table 1). However, 25 (307/1226) and 7% (50/692) of the FISH-identified A549 and SUIT-2 chromosomes had abnormalities. The chromosomes of both aneuploid lines had significantly more FISH-identified abnormalities than the diploid CCD-34Lu chromosomes (p>0.001; Table 1), and the A549 chromosomes had significantly more structural abnormalities than the SUIT-2 chromosomes (p<0.001; Fig 3A and Fig 3B; Table 1).



View larger version (29K):
[in this window]
[in a new window]
 
Figure 3. Average percentages of FISH-identified chromosome abnormalities per individual chromosome in (A) A549 and (B) SUIT-2 lines. (C) Correlation plots of the percentages of abnormalities and the % CVs (D) of these chromosome abnormalities for the individual A549 and SUIT-2 chromosomes.


 
View this table:
[in this window]
[in a new window]
 
Table 1. Percent abnormalities for FISH-identified chromosomes in CCD-34Lu, A549, and SUIT-2 karyotypes

The percentages of the different types of chromosome abnormalities for each SUIT-2 and A549 chromosome (1–22 X,Y) are plotted in Fig 3A and Fig 3B. Black-and-white hatched bars give the percent of extrachromosomal fragments (ECFs; Fig 1Ea); gray bars give the percent of chromosome breaks (Fig 1Eb; usually occurring around the centromeric regions) plus the percent of abnormalities near the telomeric regions called ENDs (Fig 1Ec), which are often hard to distinguish from breaks. Black bars give the percent of chromosomes with fusions (Fig 1Ed). Fig 3A and Fig 3B show that the highest frequencies of chromosomal abnormalities did not occur in the same FISH-identified A549 and SUIT-2 chromosomes. For example, 41% of the A549 chromosome 19s had abnormalities, whereas only 1% of the SUIT-2 chromosome 19s were abnormal (Fig 3A and Fig 3B).

To further analyze this point, Fig 3C shows the percentage of abnormalities of the individual SUIT-2 chromosomes (1–22, X,Y) on the X-axis plotted against those found in the A549 line for the same chromosomes on the Y-axis. It is apparent that there is no correlation (r=0.072) between the occurrence of FISH-identified structural abnormalities in the same individual chromosomes of the two lines. To determine whether or not the same A549 and SUIT-2 chromosomes might have highly variable frequencies of structurally abnormal chromosomes from karyotype to karyotype, we plotted the percent CVs of the chromosome abnormalities for each individual SUIT-2 (X-axis) and A549 (Y-axis) chromosome in Fig 3D. Again, there was no correlation (r=0.26) between the variability of anomalous individual chromosomes for the two aneuploid lines (Fig 3D).

DAPI-stained vs FISH-identified Chromosome Distributions
Multiple slides of each line were scanned to find karyotypic spreads suitable for simultaneous counting of the number of DAPI-stained chromosomes and chromosome-specific centromeric and paint FISH probes (Fig 1A–1C). Even after "hypo" treatment, certain karyotypes still had overlapping chromosomes, making them unsuitable for analysis. Only 90 (338/375), 98 (636/650), and 58% (378/648) of the CCD-34Lu, A549, and SUIT-2 karyotypes, respectively, were sufficiently spread for the counting of their individual DAPI-stained chromosome numbers. The mean chromosome numbers ± % CV for the DAPI-stained, CCD-34Lu, A549, and SUIT-2 karyotypes were 46 ± 1.3%, 62 ± 7%, and 76 ± 9%, respectively, and differed significantly from one another (p<0.001; Table 2). The six CCD-34Lu karyotypes that had fewer than 46 DAPI-stained chromosomes (38, 41, 42, 43, 44, and 45) were probably due to part of these karyotypes being washed off the slide during cytogenetic preparation. Fig 4A–4C show the DAPI-stained karyotypic chromosome numbers of the CCD-34Lu, A549, and SUIT-2 lines, respectively. The degrees of spread of these three DAPI-stained chromosome number distributions differ significantly from one another (Fig 4A–4C. p<0.001; Table 3). These line-specific differences in the spreads of the karyotypic chromosome number distributions (Fig 4A–4C) were not due to the introduction of bias by the selection of "evaluable karyotypes," because exactly the same results were obtained for image analysis measurement of the DNA contents (Feulgen) of 100 consecutive, intact metaphase cells of each line (p<0.001; Nestor and Allison, unpublished data).



View larger version (19K):
[in this window]
[in a new window]
 
Figure 4. DAPI-stained and "FISH-pseudo" karyotypic chromosome distributions. DAPI-stained chromosome counts of the CCD-34Lu (A), A549 (B), and SUIT-2 (C) cell lines. "FISH-pseudo" karyotypic distributions for the CCD-34Lu (D), A549 (E), and SUIT-2 (F) lines.


 
View this table:
[in this window]
[in a new window]
 
Table 2. Mean numbers of DAPI-stained and "FISH-pseudo" karyotypic chromosome distributions: mean number of DAPI-stained chromosomes


 
View this table:
[in this window]
[in a new window]
 
Table 3. Probabilities that the spreads of the DAPI- and "FISH-pseudo" karyotypic chromosome distributions differ from each othera

The numbers of FISH-identified individual chromosomes counted in the different karyotypes of each line were randomly combined into "FISH-pseudo" karyotypic chromosome distributions (see Materials and Methods). The mean chromosome numbers (± % CVs) of the "FISH-pseudo" karyotypic chromosome distributions were 46 ± 0.43%, 69 ± 4.7%, and 80 ± 4.4% for the CCD-34Lu, A549 and SUIT-2 lines, respectively (Fig 4D–4F). The diploid CCD-34Lu line showed a perfect correspondence of its DAPI-stained and "FISH-pseudo" karyotypic chromosome distributions (p=NS; Fig 3A and Fig 3D; Table 2 and Table 3). In contrast, both of the aneuploid "FISH-pseudo" karyotypic distributions had higher mean chromosome numbers and less spread than their corresponding DAPI-stained karyotypic chromosome distributions (p<0.001; Fig 4B, Fig 4E, Fig 4C, and Fig 4F; Table 2 and Table 3). Moreover, both aneuploid "FISH-pseudo" karyotypic chromosome distributions (Fig 4E and Fig 4F) had significantly more dispersion than that of the CCD-34Lu "FISH-pseudo" karyotypic distribution (p<0.001; Fig 4D; Table 3) but not from each other (p=NS; Fig 4E and Fig 4F; Table 3).


  Discussion
Top
Summary
Introduction
Materials and Methods
Results
Discussion
Literature Cited

In 1890, Hansemann observed unbalanced mitoses in human cancer cells (Hansemann 1890 ). In 1902, Boveri noted that "multipolar mitoses might lead to ... tumor-like formations" in sea urchin embryos and in 1914 presented his famous hypothesis that cancer may be due to abnormal chromosomes (Boveri 1902 ,1964, Boveri 1914 , Boveri 1929 ). Karyotypic chromosome analyses in the 1950s revealed that nontransformed human cells had a tightly regulated "diploid (2C)" number of 46 chromosomes and, in support of Boveri's hypothesis, that many cancers often had nondiploid chromosome numbers and abnormally formed chromosomes or "aneuploid" chromosomal compositions (Hsu and Moorhead 1956 ; Levan 1956 ; Makino 1956 ).

The direct examination of the cancer chromosomes of a solid tumor to determine its "ploidy level," or whether it has a diploid or aneuploid chromosome complement, is a very tedious and time-consuming procedure, requiring the establishment of a separate tissue culture line for each tumor to be karyotyped.

Measurement of the DNA contents of interphase cells by image (Swift 1950a , Swift 1950b ; Bedi and Goldstein 1976 ; Allison et al. 1981 , Allison et al. 1984 ; Hardie et al. 2002 ) or flow cytometry (Van Dilla et al. 1969 ; Kraemer et al. 1971 ; Crissman and Tobey 1974 ) allows estimates of cancer ploidy levels to be made without karyotyping. In both methods, the tumor cell DNA index is calculated as the ratio of the DNA content of the G0/G1 tumor cells to that of the diploid peak of the cells of the nontransformed tumor stroma. Although cytometric image and flow DNA measurements are subject to serious errors if performed incorrectly (Allison et al. 1984 ; Bose et al. 1989 , Bose et al. 1993 ), extensive studies with these techniques allow some firm conclusions to be drawn about the role of tumor ploidy levels in human cancer.

Most interestingly, although one might suppose that patients with aneuploid tumors (DNA index !=1) would prove to have worse prognoses than patients with diploid tumors (DNA index =1), this is not always the case. Many clinically benign tumors have aneuploid DNA contents (Anniko et al. 1984 ; van den Ingh et al. 1985 ; Joensuu et al. 1986 , Joensuu et al. 1989 ; Joensuu and Klemi 1988 ). Surprisingly, for certain infant neuroblastomas, aneuploidy in a tumor is a favorable prognostic sign (Christiansen and Lampert 1988 ; Taylor et al. 1988 ). The finding of aneuploidy in thyroid, gallbladder, and node-positive breast carcinomas gives little independent prognostic information (Hedley et al. 1987 ; Hamming et al. 1988 ; Donohue et al. 1990 ). Aneuploidy in colorectal carcinomas (Armitage et al. 1985 ; Scott et al. 1987 ; Jones et al. 1988 ; Heimann et al. 1990 ), melanoma (Kheir et al. 1988 ), and node-negative breast cancers (Clark et al. 1989 ; Ellis et al. 1989 ) is a negative prognostic indicator and is of clinical value in the selection of adjuvant therapy. The finding of aneuploidy in a pancreatic carcinoma forebodes an ominous prognosis (Allison et al. 1991 , Allison et al. 1998 ; Eskelinen et al. 1991 ).

This highly variable influence of the DNA index on patient prognosis raises the possibility that chromosomal aneuploidy is not fundamental to the genetic instability of cancer. Early molecular and karyotypic analyses appeared to support this possibility. Specifically, it was found that although karyotypic anomalies were usually highly variable in similarly staged cancers (Braun 1969 ; DiPaolo 1975 ; Harnden and Taylor 1979 ; Sandberg 1990 ; Heim and Mitelman 1995 ; Lodish et al. 1995 ; Johansson et al. 1996 ), all cells in certain cancers occasionally had somatic mutations in, or losses of, a rapidly expanding number of newly described "oncogenes" or "tumor suppressor genes" (Pitot 1986 ; Stanbridge 1990 ; Lodish et al. 1995 ; Mitelman et al. 1997 ; Haber and Fearon 1998 ; Lewin 2000 ). This suggested that aneuploidy might be a secondary event after the molecular changes that cause transformation and might play little or no role in malignant progression (Harnden and Taylor 1979 ; Cairns 1981 ; Hieter and Griffiths 1999 ).

However, as the molecular networks governing the cell cycle, DNA repair, apoptosis, and mitosis have become more clearly defined, it is apparent that the genetic defects associated with malignancy occur in thousands of genes (Stoler et al. 1999 ). Furthermore, the cancer-associated genetic changes vary from tumor to tumor, and precise and reproducible genetic defects in relatively few molecules have not been found as singular causation factors for any class of cancer (Augenlicht et al. 1987 ; Stanbridge 1990 ; Strauss 1992 ; Plattner et al. 1996 ; Heppner and Miller 1998 ; Boland and Ricciardiello 1999 ; Weitzman and Yaniv 1999 ; Duesberg et al. 2000 ; Li et al. 2000 ). The important question appears to be how cancer cells generate this wide range of genetic diversity (Strauss 1992 ; Boland and Ricciardiello 1999 ).

Aneuploidy in itself may influence genetic expression by several diverse mechanisms, including rearrangements of genetic control elements causing inappropriate gene expression, abnormal "fusion proteins" resulting from rearranged coding sequences, changes in the acetylation and/or phosphorylation of the chromatin-associated proteins altering mRNA transcription and editing, altered DNA methylation influencing patterns of gene transcription, and gene dosage effects either silencing or activating genetic expression (Klein 1994 ; Scheid et al. 1996 ; Galitski et al. 1999 ; Hieter and Griffiths 1999 ).

Several recent lines of evidence strongly suggest that aneuploidy is responsible for or associated with the genetic instability of most cancers. Only 10% of colon cancers have defects in the excision repair of the single-stranded DNA mismatch errors that cause their genetic instability. Such cancers have microsatellite instability ("MIN cancers"). Most importantly, the MIN colon cancers were found to have diploid chromosome compositions, whereas all of the MIN-negative colon cancers were aneuploid (Lengauer et al. 1997 ; Cahill et al. 1998 ), implying that chromosomal aneuploidy is in some way responsible for, or associated with, the genetic instability of the vast majority of colon cancers. Supporting this view is the recent finding of Duesberg et al. 2000 that aneuploidy invariably precedes transformation in carcinogen-treated Chinese hamster embryo cells.

Although these studies suggest that aneuploidy causes or is associated with the genetic instability of many cancers, it is still not clear why aneuploidy is such a highly variable prognostic marker for different tumors. We postulate that the wide spectrum of clinical aggressiveness among different aneuploid cancers is due to the existence of different types of cancer aneuploidy, each created by various molecular defects in gene networks governing the cell cycle, recombination, the repair of double-stranded DNA breaks, and the mitotic checkpoints.

For example, aneuploid cells are usually formed by a 2C to 4C chromosome doubling preceding chromosome losses or gains by nondisjunction of individual sister chromatid pairs or the formation of multipolar mitosis, both of which lead to daughter cells with aneuploid chromosome complements (Boveri 1902 , 1964, Boveri 1914 ; Shackney et al. 1989 ; Levine et al. 1991 ). This initial 2C to 4C chromosome doubling could be due to genetic changes in several gene networks that control the passage through mitosis (reviewed in Allison et al. 2003 ), and the specific mitotic control changes present in a given tumor may influence its subsequent mechanisms and rate of chromosome losses or gains. Similarly, molecular defects in the G1/S checkpoint allow certain cancer cells to enter S-phase without having synthesized adequate nucleotide pools to complete DNA synthesis (Allison et al. 1985 , Allison et al. 1986 , Allison et al. 1989 ; Paulovich et al. 1997 ), leading to stalled replication forks and to double-stranded DNA breaks and broken chromosomes (Paulovich et al. 1997 ). If these cancers also have genetic defects in their DNA damage surveillance and repair networks (Rouse and Jackson 2002 ), the double-stranded DNA breaks may form abnormal aneuploid chromosomes (Fig 1E) (Paulovich et al. 1997 ). Therefore, the specific defects in the G1/S checkpoint and the DNA damage-repair gene networks present in a given tumor may control its rate of aneuploid chromosome formation.

Several mitotic defects can also contribute to aneuploidy. The prometaphase migration of each sister chromatid pair stops upon arrival at the metaphase plate, but the "early arrivals" wait at the plate for the "late arrivals" before anaphase begins (reviewed in Allison et al. 2003 ). This pause is controlled by the "wait anaphase" (WA) checkpoint and is regulated by the Bub, Mad, and other mitotic-spindle associated proteins that are often lost, or altered, in aneuploid cancers (Cahill et al. 1998 ; Jaffrey et al. 2000 ; Jallepalli et al. 2001 ).

The chromosome composition of an individual aneuploid karyotype is the result of a specific lineage of gradual chromosome changes occurring over many cell generations, and the overall chromosome makeup of a given aneuploid cell population is the sum of its separate karyotype lineages (Makino 1956 ; Harada et al. 1998 ). This evolution of separate karyotypic lineages is due to the cumulative accumulation of chromosome breaks, recombinations, and nondisjunctions secondary to DNA damage (Tease 1987 ), altered nucleotide metabolism (Hecht et al. 1987 ), genetic defects leading to recombination and segregation errors (Zimmering 1987 ), and abnormal centromere/kinetochore functions (Fitzgerald 1987 ; Vig 1987 ; Vig and Sandberg 1987 ; Carlson 1988 ). The interactions of these highly complex mechanisms (Vig 1987 ; Vig and Sandberg 1987 ) lead to cancer cells with extremely variable chromosome compositions (Macville et al. 1999 ), from which genetic combinations favoring tumor progression can be selected (Johansson et al. 1996 ; Hoglund et al. 2001 ; Phillips et al. 2001 ). The complexity underlying aneuploidy has led it to be modeled as a random process (Shackney et al. 1989 ; Rasnick 2002 ) rather than assuming that discrete and identifiable subtypes of aneuploidy might exist.

Our findings suggest, however, that the chromosome compositions of a given aneuploid cell population may not occur entirely by chance. Specifically, if the mitotic, cell cycle, and DNA repair mishaps that produce aneuploidy were truly random and the same for all cancers, then the chromosomal compositions of aneuploid cell lines in long-term culture would become more similar from repeated random DNA replication and segregation errors. However, the long-term aneuploid A549 and SUIT-2 cancer lines differ significantly from each other in their DAPI-stained karyotypic chromosome numbers (Fig 1B and Fig 1C), numbers of FISH-detected individual chromosomes (Fig 2A and Fig 2B) and, most markedly, in the occurrence of FISH-detected chromosome abnormalities (p<0.001; Fig 3A and Fig 3B; Table 1 Table 2 Table 3). There was only a weak correlation between the numbers and variability of the FISH-identified individual chromosomes (Fig 2C and Fig 2D) and there was no correlation between the occurrence of FISH-identified chromosome abnormalities for the two aneuploid lines (Fig 3C and Fig 3D).

The differences between the two aneuploid lines are consistent with the idea that their overall chromosome compositions were created by differing genetic defects in their respective cell cycle, DNA repair, and mitotic checkpoint mechanisms rather than by identical and random nondisjunctions, chromosome breaks, and recombinations. For example, the higher proportion of structurally abnormal A549 chromosomes, compared to SUIT-2 chromosomes (Fig 2A and Fig 2B; Table 1) may be due to more serious defects in the A549 line's cell cycle and DNA damage checkpoints responsible for preventing abnormal chromosome formation compared to the SUIT-2 line. A549 metaphase cells with large numbers of abnormally formed chromosomes may, in turn, have difficulty in achieving sufficient numbers of bipolar microtubule attachments and/or chromosomes properly aligned at the metaphase plate necessary to trigger anaphase. If the majority of these chromosomally aberrant, metaphase-blocked A549 cells eventually die, this may explain the overall more narrowly distributed A549 karyotypic chromosome number compared to the SUIT-2 karyotypic chromosome distribution (Fig 4B and Fig 4C; Table 2 and Table 3).

Several comparative genomic hybridization (CGH) studies have found changes in the copy numbers of different chromosomes for breast, head and neck, liver and colorectal cancers (Bockmuhl et al. 1998 ; Korn et al. 1999 ; Gray et al. 2000 ; Jain et al. 2001 ). Although various selective pressures in these diverse tissue microenvironments may contribute to these tissue-specific chromosome alterations, these results are also consistent with different pathways being favored for producing chromosomal instability during the transformation of different tissue types. Supporting this possibility is a recent CGH study of hepatoblastomas from white and Japanese patients, in whom clear differences in copy numbers of chromsome13q were found, indicating that the genetic compositions of the nontransformed parental cells can influence tumor chromosome compositions in a nonrandom manner (Gray et al. 2000 ). Further, the recently reported interactions between p53 mutations and CGH changes affecting the prognosis of breast cancer patients (Jain et al. 2001 ) are also consistent with a nonrandom complexity in the gene networks that govern chromosomal instability.

Finally, random combinations of the individual FISH-identified chromosome numbers did not reconstitute the DAPI-stained karyotypic chromosome distributions of either aneuploid line (Fig 4B, Fig 4E, Fig 4C, and Fig 4F; Table 2 and Table 3): The "FISH-pseudo" distributions of both aneuploid lines had significantly higher and more tightly distributed chromosome numbers than the actual counts of their DAPI-stained aneuploid chromosomes (p<0.001; Table 2 and Table 3). The higher chromosome numbers of the "FISH-pseudo" distributions are most likely due to fusion chromosomes carrying multiple copies of FISH-detected, chromosome-specific DNA sequences (Fig 1E, Fig 3A, and Fig 3B), because fusions lower the numbers of the DAPI-stained chromosomes relative to the numbers of FISH probes detected (Table 2). The increased spreads of the DAPI-stained chromosome distributions of both aneuploid lines, relative to their "FISH-pseudo" distributions (Fig 4B, Fig 4E, Fig 4C, and Fig 4F; Table 3) is unexplained but may be because many of the counted DAPI-stained chromosomes did not have FISH-identifiable DNA sequences. Such chromosomes could undergo normal mitotic segregation by tumor activation of "neocentromeres" (reviewed in Craig et al. 1999 ) or, alternatively, such DNA fragments might be partitioned into the daughter chromosomal masses by nonmitotic mechanisms. We are now trying to determine which of these possibilities is actually occurring.

In summary, if the striking differences in chromosome compositions of the CCD-34Lu, A549, and SUIT-2 lines prove not to be rare exceptions, but the general case, then strong evidence will be provided for various genetic defects in the cell cycle, DNA repair, and mitotic checkpoints governing the chromosomal compositions of aneuploid cancers. Such heterogeneity in the genetic mechanisms governing chromosome and genome stability may provide an explanation for the wide spectrum of clinical aggressiveness of different aneuploid cancers.


  Footnotes

1 These authors contributed equally to this work.
2 Present address: Department of Surgery, Teikyo University, Tokyo, Japan.


  Acknowledgments

Supported by the Cancer Biology Fund of the Medical College of Ohio Foundation and by the F.M. Douglass Foundation, grant # 01-215, and by St. Vincent Mercy Medical Center.

We thank Kay Langenderfer for her help and support in the preparation of this manuscript and Prof Sadik Khuder for help with the statistical analysis.

Received for publication February 13, 2003; accepted May 22, 2003.


  Literature Cited
Top
Summary
Introduction
Materials and Methods
Results
Discussion
Literature Cited

Allison DC, Anderson S, Ridolpho PF, Meyne J, Robertson J (1986) Alterations in the DNA metabolism of MCa-11 mouse mammary tumor cells grown in vivo and in vitro. Cancer Res 46:3951-3957[Abstract]

Allison DC, Bose KK, Anderson S, Curley S, Robertson J (1989) Slowing of cell cycle traverse for cells in exponential monolayer cultures placed into plateau-fed and starved medium. Cancer Res 49:1456-1464[Abstract]

Allison DC, Bose KK, Hruban RH, Piantadosi S, Dooley WC, Boitnott JK, Cameron JL (1991) Pancreatic cancer cell DNA content correlates with long-term survival after pancreatoduodenectomy. Ann Surg 214:648-656[Medline]

Allison DC, Nestor AL (1999) Evidence for a relatively random array of human chromosomes on the mitotic ring. J Cell Biol 145:1-14[Abstract/Free Full Text]

Allison DC, Nestor AL, Isaka T (2003) Chromosomes during cell division. In Cooper DN, Thomas N, eds. Encyclopedia of the Human Genome. London, Nature Publishing Group

Allison DC, Lawrence GN, Ridolpho PF, O'Grady BJ, Rasch RW, Rasch EM (1984) Increased accuracy and speed of absorption cytometric DNA measurements by automatic corrections for nuclear darkness. Cytometry 5:217-227[Medline]

Allison DC, Piantadosi S, Hruban RH, Dooley WC, Fishman EK, Yeo CJ, Lillemoe KD et al. (1998) DNA content and other factors associated with ten-year survival after resection of pancreatic carcinoma. J Surg Oncol 67:151-159[Medline]

Allison DC, Ridolpho PF, Anderson S, Bose K (1985) Variations in the [3H]thymidine labeling of S-phase cells in solid mouse tumors. Cancer Res 45:6010-6016[Abstract]

Allison DC, Ridolpho PF, Rasch EM, Rasch RW, Johnson TS (1981) Increased accuracy of absorption cytophotometric DNA values by control of stain intensity. J Histochem and Cytochem 29:1219-1228[Abstract]

Anniko M, Tribukait B, Wersall J (1984) DNA ploidy and cell phase in human pituitary tumors. Cancer 53:1708-1713[Medline]

Armitage NC, Robins RA, Evans DF, Turner DR, Baldwin RW, Hardcastle JD (1985) The influence of tumour cell DNA abnormalities on survival in colorectal cancer. Br J Surg 72:828-830[Medline]

Augenlicht LH, Wahrman MZ, Halsey H, Anderson L, Taylor J, Lipkin M (1987) Expression of cloned sequences in biopsies of human colonic tissue and in colonic carcinoma cells induced to differentiate in vitro. Cancer Res 47:6017-6021[Abstract]

Bedi KS, Goldstein DJ (1976) Apparent anomalies in nuclear Feulgen-DNA contents. Role of systematic microdensitometric errors. J Cell Biol 71:68-88[Abstract]

Bockmuhl U, Wolf G, Schmidt S, Schwendel A, Jahnke V, Dietel M, Petersen I (1998) Genomic alterations associated with malignancy in head and neck cancer. Head Neck 20:145-151[Medline]

Boland CR, Ricciardiello L (1999) How many mutations does it take to make a tumor? Proc Natl Acad Sci USA 96:14675-14677[Free Full Text]

Bose KK, Allison DC, Hruban RH, Piantadosi S, Zahurak M, Dooley WC, Lin P et al. (1993) A comparison of flow cytometric and absorption cytometric DNA values as prognostic indicators for pancreatic carcinoma. Cancer 71:691-700[Medline]

Bose KK, Curley S, Smith WJ, Allison DC (1989) Differences in the flow and absorption cytometric DNA distributions of mouse hepatocytes and tumor cells. Cytometry 10:388-393[Medline]

Boveri T (1902,1964) On multipolar mitoses as a means of analysis of the cell nucleus. In Willer B, Oppenheimer J, eds. Foundations of Experimental Embryology. Englewood Cliffs, NJ, Prentice Hall, 74–97

Boveri T (1914) Zur Frae der Entshehung maligner Tumoren. Jena, Gustav Fischer-Verlag

Boveri T (1929) The Origin of Malignant Tumors. Translated by Marcella Boveri. Baltimore, Williams & Wilkins

Braun AC (1969) The Cancer Problem. A Critical Analysis and Modern Synthesis. New York, Columbia University Press

Cahill DP, Lengauer C, Yu J, Riggins GJ, Willson JK, Markowitz SD, Kinzler KW, Vogelstein B (1998) Mutations of mitotic checkpoint genes in human cancers. Nature 392:300-303[Medline]

Cairns J (1981) The origin of human cancers. Nature 289:353-357[Medline]

Carlson WR (1988) Chromosomes as a model system for nondisjunction. In Vig BK, Sandberg AA, eds. Aneuploidy, Part B: Induction and Test Systems. New York, Alan R Liss, 199-207

Christiansen H, Lampert F (1988) Tumour karyotype discriminates between good and bad prognostic outcome in neuroblastoma. Br J Cancer 57:121-126[Medline]

Clark GM, Dressler LG, Owens MA, Pounds G, Oldaker T, McGuire WL (1989) Prediction of relapse or survival in patients with node-negative breast cancer by DNA flow cytometry. N Eng J Med 320:627-633[Abstract]

Craig JM, Earnshaw WC, Vagnarelli P (1999) Mammalian centromeres: DNA sequence, protein composition, and role in cell cycle progression. Exp Cell Res 246:249-262[Medline]

Crissman HA, Tobey RA (1974) Cell-cycle analysis in 20 minutes. Science 184:1297-1298[Medline]

DiPaolo JA (1975) Karyological instability of neoplastic somatic cells. In Vitro 11:89-96[Medline]

Donohue JH, Nagorney DM, Grant CS, Tsushima K, Ilstrup DM, Adson MA (1990) Carcinoma of the gallbladder. Does radical resection improve outcome? Arch of Surg 125:237-241

Duesberg P, Li R, Rasnick D, Rausch C, Willer A, Kraemer A, Yerganian G, Hehlmann R (2000) Aneuploidy precedes and segregates with chemical carcinogenesis. Cancer Genet Cytogenet 119:83-93[Medline]

Ellis CN, Frey ES, Burnette JJ, Akin JMJ, Reading C, Gaskin TA, Blakemore WS (1989) The content of tumor DNA as an indicator of prognosis in patients with T1N0M0 and T2N0M0 carcinoma of the breast. Surgery 106:133-138[Medline]

Eskelinen M, Lipponen P, Collan Y, Marin S, Alhava E, Nordling S (1991) Relationship between DNA ploidy and survival in patients with exocrine pancreatic cancer. Pancreas 6:90-95[Medline]

Fitzgerald PH (1987) Premature centromeric division and aneuploidy. In Vig BK, Sandberg AA, eds. Aneuploidy, Part A: Incidence and Etiology. New York, Alan R Liss, 249-264

Galitski T, Saldanha AJ, Styles CA, Lander ES, Fink GR (1999) Ploidy regulation of gene expression. Science 285:251-254[Abstract/Free Full Text]

Gray SG, Kytola S, Matsunaga T, Larsson C, Ekstrom TJ (2000) Comparative genomic hybridization reveals population-based genetic alterations in hepatoblastomas. Br J Cancer 83:1020-1025[Medline]

Haber DA, Fearon ER (1998) The promise of cancer genetics. Lancet 351(suppl 2):SII1-8[Medline]

Hamming JF, Schelfhout LJ, Cornelisse CJ, van de Velde CJ, Goslings BM, Hermans J, Fleuren GJ (1988) Prognostic value of nuclear DNA content in papillary and follicular thyroid cancer. World J Surg 12:503-508[Medline]

Hansemann D (1890) Ueber asymmetrische Zelltheilung en Epithelkrebsen und deren biologische Bedeutung. Virchows Arch 119:229-326. [A]

Harada K, Nishizaki T, Ozaki S, Kubota H, Ito H, Sasaki K (1998) Intratumoral cytogenetic heterogeneity detected by comparative genomic hybridization and laser scanning cytometry in human gliomas. Cancer Res 58:4694-4700[Abstract]

Hardie DC, Gregory TR, Hebert PDN (2002) From pixels to picograms: a beginners' guide to genome quantification by Feulgen image analysis densitometry. J Histochem Cytochem 50:735-749[Abstract/Free Full Text]

Harnden DG, Taylor AM (1979) Chromosomes and neoplasia. In Harris H, Hirschhorn K, eds. Advances in Human Genetics. Vol 9. New York, Plenum Press, 1-70

Hecht F, Defendi GL, Bixenman HA, Hecht BK (1987) Human aneuploidy and folic acid deficiency. In Vig BK, Sandberg AA, eds. Aneuploidy, Part A: Incidence and Etiology. New York, Alan R Liss, 159-162

Hedley DW, Rugg CA, Gelber RD (1987) Association of DNA index and S-phase fraction with prognosis of nodes positive early breast cancer. Cancer Res 47:4729-4735[Abstract]

Heim S, Mitelman F (1995) Cancer Cytogenetics. New York, Wiley-Liss

Heimann TM, Miller F, Martinelli G, Mester J, Kurtz RJ, Szporn A, Fasy T (1990) Significance of DNA content abnormalities in small rectal cancers. Am J Surg 159:199-202[Medline]

Heppner GH, Miller FR (1998) The cellular basis of tumor progression. Int Rev Cytol 177:1-56[Medline]

Hieter P, Griffiths T (1999) Polyploidy—more is more or less. Science 285:210-211[Free Full Text]

Hoglund M, Sall T, Heim S, Mitelman F, Mandahl N, Fadl–Elmula I (2001) Identification of cytogenetic subgroups and karyotypic pathways in transitional cell carcinoma. Cancer Res 61:8241-8246[Abstract/Free Full Text]

Hsu T, Moorhead P (1956) Chromosome anomalies in human neoplasms with special reference to the mechanisms of polyploidization and aneuploidization in the HeLa strain. Ann NY Acad Sci 63:1083-1094

Jaffrey RG, Pritchard SC, Clark C, Murray GI, Cassidy J, Kerr KM, Nicolson MC et al. (2000) Genomic instability at the BUB1 locus in colorectal cancer, but not in non-small cell lung cancer. Cancer Res 60:4349-4352[Abstract/Free Full Text]

Jain AN, Chin K, Borresen–Dale AL, Erikstein BK, Eynstein Lonning P, Kaaresen R, Gray JW (2001) Quantitative analysis of chromosomal CGH in human breast tumors associates copy number abnormalities with p53 status and patient survival. Proc Natl Acad Sci USA 98:7952-7957[Abstract/Free Full Text]

Jallepalli PV, Waizenegger IC, Bunz F, Langer S, Speicher MR, Peters JM, Kinzler KW et al. (2001) Securin is required for chromosomal stability in human cells. Cell 105:445-457[Medline]

Joensuu H, Klemi PJ (1988) DNA aneuploidy in adenomas of endocrine organs. Am J Pathol 132:145-151[Abstract]

Joensuu H, Klemi PJ, Alanen KA (1989) Co-existence of two aneuploid stemlines in benign adenomas. A report of three cases with stemline heterogeneity. Virchows Arch 415:175-180. [A]

Joensuu H, Klemi P, Eerola E (1986) DNA aneuploidy in follicular adenomas of the thyroid gland. Am J Pathol 124:373-376[Abstract]

Johansson B, Mertens F, Mitelman F (1996) Primary vs. secondary neoplasia-associated chromosomal abnormalities—balanced rearrangements vs. genomic imbalances? Genes Chromosomes Cancer 16:155-163[Medline]

Jones DJ, Moore M, Schofield PF (1988) Prognostic significance of DNA ploidy in colorectal cancer: a prospective flow cytometric study. Br J Surg 75:28-33[Medline]

Kheir SM, Bines SD, Vonroenn JH, Soong SJ, Urist MM, Coon JS (1988) Prognostic significance of DNA aneuploidy in stage I cutaneous melanoma. Ann Surg 207:455-461[Medline]

Klein G (1994) Roles of the myc gene in cell proliferation and differentiation, as deduced from its role in tumorigenesis. In Gordon S, ed. The Legacy of Cell Fusion. Oxford, UK, Oxford University Press, 261-269

Korn WM, Yasutake T, Kuo WL, Warren RS, Collins C, Tomita M, Gray J et al. (1999) Chromosome arm 20q gains and other genomic alterations in colorectal cancer metastatic to liver, as analyzed by comparative genomic hybridization and fluorescence in situ hybridization. Genes Chromosomes Cancer 25:82-90[Medline]

Kraemer PM, Petersen DF, Van DMA (1971) DNA constancy in heteroploidy and the stem line theory of tumors. Science 174:714-717[Medline]

Lengauer C, Kinzler KW, Vogelstein B (1997) Genetic instability in colorectal cancers. Nature 386:623-627[Medline]

Levan A (1956) Chromosomes in cancer tissue. Ann NY Acad Sci 63:774-794

Levine DS, Sanchez CA, Rabinovitch PS, Reid BJ (1991) Formation of the tetraploid intermediate is associated with the development of cells with more than four centrioles in the elastase-simian virus 40 tumor antigen transgenic mouse model of pancreatic cancer. Proc Natl Acad Sci USA 88:6427-6431[Abstract]

Lewin B (2000) Oncogenes and cancer. In Genes VII. New York, Oxford University Press, 875–912

Li R, Sonik A, Stindl R, Rasnick D, Duesberg P (2000) Aneuploidy vs. gene mutation hypothesis of cancer: recent study claims mutation but is found to support aneuploidy. Proc Natl Acad Sci USA 97:3236-3241[Abstract/Free Full Text]

Lodish H, Baltimore D, Berk A, Zipursky SL, Matsudaira P, Darnell J (1995) Cancer. In Molecular Cell Biology. , ed. New York. American Scientific Books, 1, 247-1294

Macville M, Schrock E, Padilla-Nash H, Keck C, Ghadimi BM, Zimonjic D, Popescu N et al. (1999) Comprehensive and definitive molecular cytogenetic characterization of HeLa cells by spectral karyotyping. Cancer Res 59:141-150[Abstract/Free Full Text]

Makino S (1956) Further evidence favoring the concept of the stem cell in ascites tumors of rats. Ann NY Acad Sci 63:818-830

Mitelman F, Mertens F, Johansson B (1997) A breakpoint map of recurrent chromosomal rearrangements in human neoplasia. Nature Genet 15(spec no):417-474[Medline]

Nestor AL, Willey J, Allison DC (2001) Tissue culture, cell growth, and analysis. In Souba WW, Wilmore DW, eds. Surgical Research. San Diego, Academic Press, 193-206

Nurse P (1997) Checkpoint pathways come of age. Cell 91:865-867[Medline]

Nurse P (2000) A long twentieth century of the cell cycle and beyond. Cell 100:71-78[Medline]

Paulovich AG, Toczyski DP, Hartwell LH (1997) When checkpoints fail. Cell 88:315-321[Medline]

Phillips JL, Hayward SW, Wang Y, Vasselli J, Pavlovich C, Padilla–Nash H, Pezullo JR et al. (2001) The consequences of chromosomal aneuploidy on gene expression profiles in a cell line model for prostate carcinogenesis. Cancer Res 61:8143-8149[Abstract/Free Full Text]

Pitot HC (1986) Fundamentals of Oncology. 3rd ed New York, Marcel Dekker, pp. 95–314

Plattner R, Anderson MJ, Sato KY, Fasching CL, Der CJ, Stanbridge EJ (1996) Loss of oncogenic ras expression does not correlate with loss of tumorigenicity in human cells. Proc Natl Acad Sci USA 93:6665-6670[Abstract/Free Full Text]

Rasnick D (2002) Aneuploidy theory explains tumor formation, the absence of immune surveillance, and the failure of chemotherapy. Cancer Genet Cytogenet 136:66-72[Medline]

Rouse J, Jackson SP (2002) Interfaces between the detection, signaling, and repair of DNA damage. Science 297:547-551[Abstract/Free Full Text]

Sandberg AA (1990) The Chromosomes in Human Cancer and Leukemia. New York, Elsevier Science

Scheid OM, Jakovleva L, Afsar K, Maluszynska J, Paszkowski J (1996) A change of ploidy can modify epigenetic silencing. Proc Natl Acad Sci USA 93:7114-7119[Abstract/Free Full Text]

Scott NA, Wieand HS, Moertel CG, Cha SS, Beart RW, Lieber MM (1987) Colorectal cancer. Dukes' stage, tumor site, preoperative plasma CEA level, and patient prognosis related to tumor DNA ploidy pattern. Arch Surg 122:1375-1379

Shackney SE, Smith CA, Miller BW, Burholt DR, Murtha K, Giles HR, Ketterer DM et al. (1989) Model for the genetic evolution of human solid tumors. Cancer Res 49:3344-3354[Abstract]

Stanbridge EJ (1990) Human tumor suppressor genes. Ann Rev Genet 24:615-657[Medline]

Stoler DL, Chen N, Basik M, Kahlenberg MS, Rodriguez–Bigas MA, Petrelli NJ, Anderson GR (1999) The onset and extent of genomic instability in sporadic colorectal tumor progression. Proc Natl Acad Sci USA 96:15121-15126[Abstract/Free Full Text]

Strauss BS (1992) The origin of point mutations in human tumor cells. Cancer Res 52:249-253[Medline]

Swift HF (1950a) The constancy of deoxyribose nucleic acid in plant nuclei. Proc Natl Acad Sci USA 36:643-654[Medline]

Swift HF (1950b) The deoxyribose nucleic acid content of animal nuclei. Physiol Zool 23:169-198

Taylor SR, Blatt J, Costantino JP, Roederer M, Murphy RF (1988) Flow cytometric DNA analysis of neuroblastoma and ganglioneuroma. A 10-year retrospective study. Cancer 62:749-754[Medline]

Tease C (1987) Radiation-induced aneuploidy in germ cells of female mammals. In Vig BK, Sandberg AA, eds. Aneuploidy, Part A: Incidence and Etiology. New York, Alan R Liss, 141-157

van den Ingh HF, Griffioen G, Cornelisse CJ (1985) Flow cytometric detection of aneuploidy in colorectal adenomas. Cancer Res 45:3392-3397[Abstract]

Van Dilla MA, Trujillo TT, Mullaney PF, Coulter JR (1969) Cell microfluorometry: a method for rapid fluorescence measurement. Science 163:1213-1214[Medline]

Vig BK (1987) Sequential centromere separation in multicentric chromosomes: relationship to aneuploidy. In Vig BK, Sandberg AA, eds. Aneuploidy, Part A: Incidence and Etiology. New York, Alan R Liss, 265-272

Vig BK, Sandberg AA (1987) Aneuploidy incidence and etiology. In Vig BK, Sandberg AA, eds. Aneuploidy, Part A: Incidence and Etiology. New York, Alan R Liss, 415-419

Weitzman JB, Yaniv M (1999) Rebuilding the road to cancer. Nature 400:401-402[Medline]

Zimmering S (1987) Aneuploidy in Drosophila. In Vig BK, Sandberg AA, eds. Aneuploidy, Part A: Incidence and Etiology. New York, Alan R Liss, 147-178





This Article
Abstract
Full Text (PDF)
Alert me when this article is cited
Alert me if a correction is posted
Citation Map
Services
Similar articles in this journal
Similar articles in PubMed
Alert me to new issues of the journal
Download to citation manager
Google Scholar
Articles by Isaka, T.
Articles by Allison, D. C.
Articles citing this Article
PubMed
PubMed Citation
Articles by Isaka, T.
Articles by Allison, D. C.


Home Help [Feedback] [For Subscribers] [Archive] [Search] [Contents]