Correlation between dysplasia and mutations of six tumor suppressor genes in Barrett's esophagus

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Original article: general thoracic

Correlation between dysplasia and mutations of six tumor suppressor genes in Barrett’s esophagus

Siva Raja, BS^a, Sydney D. Finkelstein, MD^c, Fabien K. Baksh, MD^c, William E. Gooding, MS^b, Patricia A. Swalsky, BS^c, Tony E. Godfrey, PhD^a, Percival O. Buenaventura, MD^a, James D. Luketich, MD^a

^a Division of Thoracic Surgery, Department of Surgery, University of Pittsburgh Medical Center Health System, Pittsburgh, Pennsylvania, USA
^b Department of Biostatistics, University of Pittsburgh Medical Center Health System, Pittsburgh, Pennsylvania, USA
^c Department of Pathology, University of Pittsburgh Medical Center Health System, Pittsburgh, Pennsylvania, USA

Address reprint requests to Dr Luketich, Section of Thoracic Surgery, University of Pittsburgh Medical Center, C800, PUH, 200 Lothrop St, Pittsburgh, PA 15213
e-mail: luketichjd{at}msx.upmc.edu

Presented at the Thirty-seventh Annual Meeting of The Society of Thoracic Surgeons, New Orleans, LA, Jan 29–31, 2001.

Abstract

Top
Abstract
Introduction
Material and methods
Results
Comment
Discussion
References

Background. Barrett’s esophagus (BE) may progress to adenocarcinomathrough dysplastic progression. Classification of dysplasiain BE has significant interobserver variability. Our objectivewas to determine whether genetic alterations in BE correlatewith degrees of histologic dysplasia.

Methods. Fixed tissue from 37 patients with BE and adenocarcinomawas studied for six tumor suppressor genes. Tissues were microdissectedand analyzed for loss of heterozygosity. Microdissection ofindividual crypts showing metaplasia and dysplasia were performedand analyzed for 23 of the 37 patients whose tumors were heterozygousfor at least four of the six genes studied.

Results. Frequency of alterations for MXI1, hOGG1, p53, MTS1,DCC, and APC were 7 of 32 (22%), 12 of 35 (34%), 12 of 26 (46%),17 of 30 (57%), 17 of 27 (63%), and 23 of 36 (64%), respectively.Analysis of BE demonstrated that crypts with metaplasia, low-gradedysplasia, and high-grade dysplasia strongly correlated withalterations in tumor suppressor genes (p < 0.0001).

Conclusions. This pilot study demonstrates that genetic analysiscan be performed on individual crypts in patients with BE, andthat alterations may facilitate objective classification ofthe severity of dysplasia.

Introduction

Top
Abstract
Introduction
Material and methods
Results
Comment
Discussion
References

Adenocarcinoma of the esophagus accounts for approximately 11,500deaths annually in the United States [1]. Over the past 10 yearsthere has been a dramatic increase in both the incidence andmortality from esophageal adenocarcinoma [2]. Unfortunately,most patients with esophageal cancer are diagnosed with advancedregional lymph node involvement or distant metastasis. It hasbeen demonstrated that surgical resection is most likely tobe curative when the disease is limited to only high-grade dysplasiaor a minimally invasive tumor [3]. Thus efforts to reduce mortalityhave centered on early detection of disease.

The risk of developing esophageal cancer is increased (30- to125-fold) [4] in the presence of gastroesophageal reflux disease(GERD) combined with the metaplastic transformation of the esophagealsquamous lining into glandular columnar mucosa referred to asBarrett’s metaplasia (BE) [5]. The diagnosis of BE leadsto periodic surveillance endoscopy with biopsy [4]; if progressionto high-grade dysplasia occurs, surgical resection is generallyrecommended. From a histopathologic perspective, a particularlychallenging problem is the accurate and reliable diagnosis andclassification of Barrett’s metaplasia and dysplasia.There is considerable interobserver variation, even among expertsin the field, which is compounded by the significant samplingvariation inherent in biopsy of a macroscopic field of at-riskmucosa [6]. Objective diagnosis and classification of Barrett’sdysplasia based on molecular characteristics offers the potentialto contribute to a more consistent diagnosis of high-grade dysplasia,and perhaps to determine risk factors for progression from simpleBE.

The molecular pathogenesis of cancer has been shown to resultfrom an accumulation of multiple genetic alterations in a multistepfashion over time. In esophageal cancer, loss of heterozygosityof tumor suppressor genes such as p53, APC the adenomatous polyposiscoli gene (APC), the gene deleted in colon cancer (DCC), andMTS1 (p16) have been reported in numerous previous studies [7–9].Additionally, alterations in other genes such as MXI1 (MAX interactingprotein) and human OGG1 have been implicated in other epithelialcell malignancies [10, 11]. Since adenocarcinoma of the esophagusevolves from dysplastic cells in BE, it is likely that progressionfrom metaplasia to cancer follows a predictable and quantifiablepattern of acquisition of genetic alterations. The aim of thisstudy was to determine whether loss of heterozygosity in individualcrypts of BE in the mucosa adjacent to an existing adenocarcinomawould be present in proportion to the degree of histologic dysplasia.

Material and methods

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Abstract
Introduction
Material and methods
Results
Comment
Discussion
References

Patients and specimens
All studies were conducted with the approval of the institutionalreview board of the University of Pittsburgh Medical Center(UPMC). Archived samples from 37 patients who underwent esophagealresection at UPMC for primary adenocarcinoma arising from BEbetween 1997 and 1999 were studied. Slides were reviewed andblocks selected showing carcinoma at its deepest point of invasionas well as associated Barrett’s metaplasia and dysplasiawhen present. Intestinalized crypts were selected in each caseshowing histologic features classified as metaplasia withoutdysplasia, indeterminate for dysplasia, low-grade dysplasia,and high-grade dysplasia. Eight serial 4-µm sections wereprepared to serve as a basis for microdissection genotyping.The analysis also included five examples of esophageal ulcerationand associated inflammatory change without evidence of dysplasiaand malignancy. The latter group was included to evaluate genedamage in nonneoplastic tissue.

Microdissection and DNA extraction
All microdissections were performed by the same pathologist(S.D.F.) using a stereomicroscope (Zeiss SZ-40; Zeiss, Oberkochen,Germany). Tissue extraction from formalin-fixed, paraffin-embeddedsections was performed as described previously [12] (Fig 1A and 1B).Briefly, sequential 4-µm-thick sections werecut and one was stained with hematoxylin and eosin to localizelesions of interest for microdissection. Paraffin-embedded sectionswere deparaffinized in xylene (2x3 minutes) and washed in 100%ethanol (2x3 minutes). In each case, more than 85% neoplastic(> 500 cells) and paired corresponding normal tissues were taken.Similarly, individual crypts of varying levels of dyplasia weremicrodissected over six to eight serial sections. Microdissectedtissues were incubated at 37°C overnight with 10 mg/mL proteinaseK. The products were stored at -20°C until polymerase chainreaction (PCR) amplification.

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Fig 1. (A) Hematoxylin and eosin–stained section of esophagus with microdissection of adenocarcinoma (A), crypt of Barrett’s esophagus (C), and normal skeletal muscle tissue (N). (B) Serial hematoxylin and eosin–stained sections showing crypt microdissection (arrow).

PCR amplification and DNA isolation
PCR was performed on an Omn-E thermal cycler (Hybaid, Franklin,MA) using 1 µL of genomic DNA, 10 pmol of each primer(Table 1), 300 nmol/L of deoxynucleotide triphosphates, 1.5mmol/L magnesium chloride, 0.25 U of TaqGold DNA polymerase,and 5 µL of 10xPCR buffer (Perkin Elmer Cetus, Norwalk,CT) in a final volume of 50 µL. After initial denaturationat 95°C for 10 minutes, 35 cycles PCR were carried out asfollows: denaturation at 94°C for 1 minute, annealing at58°C for 1 minute, and polymerization at 74°C for 1minute, with a final 10-minute extension at 74°C. PCR-generatedDNA was isolated through electrophoresis in 2% agarose gel.The target bands of each gene were cut from agarose gel underultraviolet light transilluminator and dissolved in 1 µLof 50xGelase buffer (Epicentre Technologies, Madison, WI) at95°C for 8 minutes, followed by incubation with 1 U of Gelaseenzyme at 45°C for 1 hour.

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Table 1. Primers Used in Study^a

Direct DNA sequencing
DNA sequencing for amplified PCR products of APC, OGG1, DCC,and p53 was performed using T7 Sequenase, Version 2.0, DNA sequencingkit (Amersham Life Science, Cleveland, OH), according to themanufacturer’s instructions. Each tumor suppressor geneexcept for MTS1 and MXI1 was originally sequenced with fourlanes (A, G, C, and T); afterward only two lanes showing thepolymorphic bands were necessary to load on the sequence gel.The upstream primers of APC, DCC, and OGG1 and the downstreamprimer of p53 (Table 1) served as the sequencing primers. Fordetecting loss of heterozygosity (LOH) in the microsatellites,aliquots of the crude lysate were added into the reaction mixture(10 µL) containing 2.5 µCi of [ ${alpha}$ -33P] dNTP (dATP,dGTP, dCTP, dTTP; New Life Science Products, Boston, MA), and0.25 µL of Ampli Taq DNA polymerase (Perkin Elmer Cetus,Norwalk, CT). These were run through 6% polyacrylamide gel electrophoresisat 2000 V for 1 to 2 hours. The gel was dried at 80°C for40 minutes on a Savant gel dryer SG210D (Savant InstrumentsInc, Holbrook, NY) and exposed overnight to Kodak X-Omat AR-2film (Eastman Kodak, Rochester, NY). The sequence was read visuallywith the use of a light box.

Definition of LOH
On an autoradiograph of the sequencing gel, heterozygosity fora locus is visualized as the presence of two bands of equalfragment size on lanes corresponding to two different nucleotides(Fig 2). Films were digitized using the Gel Doc 2000 (Bio-RadLaboratories, Hercules, CA) and densitometry was performed onthe appropriate bands and the resultant data were analyzed usingthe Quantity-one software (Bio-Rad Laboratories). LOH was determinedby the method described by MacGrogan and colleagues [13] withthe following difference. The cut off value for LOH was setat 1.4 for the ratio of ratios (based on the histogram of allthe values from all the loci in this study). The same gels werealso analyzed through subjective means by at least two differentobservers to guard against experimental artifact.

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Fig 2. Typical autoradiograph showing the loss of heterozygosity (LOH) in a pentanucleotide polymorphism from a tumor sample (right) relative to a normal sample (left) from the same patient.

Methods for crypt LOH analysis
Given the small size of the fixative treated, microdissectedmetaplastic/dysplastic intestinalized crypt samples for genotyping,preliminary steps were taken to determine the minimum amountof sample sufficient to afford balanced representative PCR therebyavoiding allelic dropout. This was done using a 5' fluorogenicassay for ß-actin and standard curve using human genomicDNA. Each microdissected sample was run against a standard derivedfrom freshly extracted DNA ranging from 0.08 to 4 ng of DNA.This was used to control the DNA input into each reaction.

Genetic analysis
The genes of interest were studied using direct DNA sequencingof intragenic sequence polymorphism or microsatellite analysis.LOH in DCC, p53, hOGG1, and APC genes were studied by both techniques.A loss at either the intragenic loci or at the associated microsatelliteloci was sufficient to determine loss of the allele. For thegenes MTS1 and MXI1 a loss in at least one of the two flankingmicrosatellite loci was sufficient to determine loss.

Results

Top
Abstract
Introduction
Material and methods
Results
Comment
Discussion
References

Esophageal adenocarcinomas were notable for the presence offrequent allelic imbalance affecting the genes studied (Table 2).The mean number of heterozygous gene loci per patient was5.05 (median 5.00) and the mean number of genes demonstratingLOH was 2.52 (median 2.00). There were three patients who didnot show any loss out of the 3, 4, and 5 heterozygous gene locirespectively. There were five samples of esophageal mucosa thatwere diagnosed as having an inflammatory appearance. These casesdid not show allelic imbalance in the genes from our panel.No single gene in our panel was found to be universally mutatedor nonmutated in esophageal cancer. Thus reliance on any singlegene to indicate the presence or absence of dysplasia or malignancycould not be established. Instead, a combination of gene targetsin the form of a panel could achieve the high degree of associationwith the process of carcinogenesis.

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Table 2. Genetic Alterations in Primary AC

Determination of amplifiable DNA using a standard curve of freshlyextracted DNA indicated that microdissection samples variedsignificantly in their respective amounts of amplifiable DNA.Although certain histologic features such as necrosis correlatedwith diminished amounts of amplifiable DNA, in many cases cellularmorphologic features could not explain the difference in DNAcontent. Thus it was necessary to determine the amount of amplifiableDNA in each microdissected sample to ensure that adequate quantitiesof DNA were present in each PCR to avoid allelic dropout [14,15]. Values of less than 100 pg yielded variable results thatcould be interpreted as loss of heterozygosity. The polymorphicmarkers used in this study varied in their requirement for minimumthreshold levels of amplifiable DNA from 40 to 100 pg of DNA.To simplify the processing of specimens, a value of 100 pg ofamplifiable DNA was applied to each PCR reaction.

Intestinalized crypts of Barrett’s esophagus were microdissectedfrom esophageal resection specimens bearing invasive adenocarcinoma.These microdissected crypts manifested cellular changes rangingfrom metaplasia without dysplasia to high-grade dysplasia. Severalobservations on this individual crypt analyses were notable.First, the mutational profile of individual crypts differedsignificantly from one another, in keeping with independentclonal expansion of mutated clones of dysplastic cells. Also,the genotype of dysplastic Barrett crypts did not necessarilymirror that of the invasive adenocarcinoma that had developedin the esophagus. The findings were consistent with a fieldeffect producing multiple independent clones of tumor cellswith one progressing more rapidly into malignancy and accountingfor the malignancy in each case. There was a close and strongcorrelation (p < 0.001, Jonckherre-Terpstra Test) betweenthe extent of allelic loss and grade of dysplasia in Barrett’sesophagus (Table 3). Intestinalized crypts showing metaplasiawithout dysplasia in all cases but one were without allelicloss. In contrast, most crypts bearing high-grade dysplasticepithelium manifest two or more different allelic loss events.Low-grade dysplasia displayed intermediate levels of mutationalchange.

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Table 3. Genotyping of Crypts in Barrett’s Esophagus

	Comment

Top Abstract Introduction Material and methods Results Comment Discussion References

The diagnosis of Barrett’s high-grade dysplasia has seriousimplications. High-grade dysplasia is currently treated by esophagectomy[16] or, in nonsurgical candidates, with ablative therapiessuch as mucosal stripping or photodynamic therapy [17]. Thisaggressive approach is taken because of the high risk for developingsubsequent adenocarcinomas or already harboring a focus of invasivecancer in the esophagus of patients with high-grade dysplasia[2]. Therefore, given this serious implication, it is vitalto make an accurate diagnosis of high-grade dysplasia for BE.Yet there is considerable interobserver variation even amongexperts in the field, which is compounded by the significantsampling variation inherent in biopsy of a macroscopic fieldof at-risk mucosa. In a study by Reid and colleagues [6], theinterobserver agreement for the diagnosis of high-grade versuslower grades of dysplasia and no dysplasia was only 86%. Furthermore,the concordance for dyplasia versus no dyplasia was even lowerat 72%. Inflammatory changes in the metaplastic mucosa can furtherconfound the distinction between reactive hyperplasia and dysplasia.The more objective diagnosis and classification of Barrett’sdysplasia based on molecular characteristics may offer the potentialfor better diagnosis and treatment planning.

Our multigene analysis of esophageal adenocarcinoma arisingin the context of Barrett’s metaplasia demonstrates astriking multiplicity of tumor suppressor gene loss. Recognizingthat the genes we selected for study of allelic loss determinationrepresent only a small proportion of known tumor suppressorgenes, it was noteworthy to find that even this limited panelof 6 markers were significantly altered in the tumor. It isclear that the panel of genes used in this study may not optimallyinclude those specific genetic targets most intimately involvedin esophageal tumorigenesis. Nevertheless, this introductorypanel can be employed to study both esophageal dysplasia andcarcinoma with the expectation that it may include useful molecularmarkers for diagnostic and prognostic purposes. Our data suggestthat molecular quantitiation of the frequency of LOH in individualintestinalized crypts can potentially be used to classify themicrodissected sample as nondysplastic, low-grade dysplasia,or high-grade dysplasia. Moreover, the indeterminate categorymay potentially be divided into true dysplasia with allelicloss versus nondysplastic crypts lacking mutational change (Table 2).The observation that increasing numbers of mutations correlatewith the degree of dysplasia in BE was highly statisticallysignificant (p < 0.0001).

Our data support the contention that loss of tumor suppressorgenes is widespread with respect to the involvement of specificgenes, that it may be expected to affect many well-characterizedgenes, and that it is not due to a single genetic alteration.This study adds strength to the current paradigm that the evolutionof this tumor from BE may not follow a linear pathway [18].It might occur through several pathways, or they could convergeonto a single pathway at a gene that has yet to be identifiedor investigated.

The creation of a panel of genes that could be used to distinguishdysplasia and tumor from benign processes would appear to besupported by our genotyping results. In our panel of six genes,with the exception of 3 cases, every patient had at least onealtered gene. We also demonstrated the feasibility for performingthis type of analysis on very small amount of tissue from microdissectedindividual columnar lined crypts. The importance of this findinglies in the potential for this type of analysis to be appliedto biopsy specimens. By demonstrating that it is possible tomicrodissect single crypts, we can specifically target thosecrypts that pose a problem for conventional histopathologicevaluation.

There are some limitations that need to be recognized. First,the amount of DNA available for analysis is small, limitingthe genotyping analysis to approximately 8 to 10 separate loci.As such, the presence of heterozygosity would need to be establishedbefore sample testing. This can be achieved by initially evaluatinggermline DNA from the cellular component of blood to establishheterozygous loci for the gene targets. Alternative gene targetswould need to be available to substitute for those loci thatprove to be homozygous for an individual patient. The resultsof this study indicate that such an approach is feasible usingthe markers employed in this analysis. With the sequencing ofthe human genome, it can be expected that additional polymorphicloci as well as new gene targets providing greater frequencyof heterozygosity with respect to esophageal cancer developmentand progression, will be part of an optimized panel of genotypingmarkers for this cancer.

The most significant aspect of this work is the strategy usedto integrate tissue histopathology and molecular genetics ofcancer for diagnostic purposes. By creating a panel of cancergene analysis, specific questions in the molecular pathogenesisof cancer can be addressed. The genotyping analysis carriedout on microdissected, fixed tissue specimens enabled precisesample selection for specific genetic testing. In this way themolecular changes underlying specific cellular events can bedefined in a manner that is both objective and especially meaningful,given the causative relationship between gene damage and carcinogenesis.The task remains to define the specific gene targets that willbe used in this regard and the best methodology enabling thegenotyping to be performed in a rapid, simple, reliable mannerwithout impeding established pathology practice. The resultsof this work provide a basis on which to pursue this objective.

Discussion

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Abstract
Introduction
Material and methods
Results
Comment
Discussion
References

DR STEVE R. DeMEESTER (Los Angeles, CA): That was a very nicepresentation.

I found it interesting that every patient had tumor, I assume,and within each patient you were able to find areas of no dysplasia,low-grade, high-grade, and the tumor itself. Often you can’teven find Barrett’s in patients with adenocarcinoma, muchless find each of those different tissues. How often could younot identify all of those different gradations of dysplasiain a patient, or were these assembled from many patients?

Additionally we have noted that there seems to be quite a fieldeffect. We have not been able to find such a disparity betweenthe genetic changes in low-grade versus high-grade dysplasiain these patients. It is more of a field effect. It is universalthroughout the tumor and the Barrett’s tissue. So I wassurprised that you found such a big difference. Is this perhapsbecause the samples are from different patients and there isa lot of variability between patients?

In addition, did you look at methylation at all? We know thatgenes can be silenced by methylation independently of loss ofthe gene. Have you looked at that?

Last, it strikes me as a little bit of a circular argument,one of your conclusions that the genetic changes may help youdetermine the degree of dysplasia, because you categorized thingsbased on dysplasia. If you’re saying that dysplasia isvariable by pathologists, yet you use dysplasia to correlateor categorize your genetic changes, that is a bit of a circularargument. How do you get around that?

Thank you.

DR RAJA: To address your first question, in fact, we rarelyfound all the levels of dysplasia within the same patient. Infact, if you look at the table, there were 11 patients withnegative dysplasia, whereas in fact 23 patients had been analyzedfor the study, and the number does not add up. That’sbecause in a given patient we could only identify a certainnumber of these alterations, maybe high-grade dysplasia onlyor high-grade dysplasia and low-grade dysplasia without anynegative dysplasia. It depends on what is available in the fieldat that time. So, in fact, we did not see all levels of dysplasiawithin the same specimen.

The second question, I do agree that it is a field effect, andin fact our data does support that hypothesis. The mutationsthat were seen in the dysplastic crypts were not necessarilythe same genes that were lost in the cancer. Oftentimes theywere, but that did not necessarily have to be the case. So webelieve that that aspect of our data supports the field effect,meaning that all the cells in the gastroesophageal junctionare exposed to the same insult and, hence, undergo similar processes.

Your third question regarding methylation, those studies arecurrently underway. And specifically one of the genes that welooked at, MTS1, also known as p16, is traditionally characterizedas having methylation inactivation, and we found that that geneappeared to be heavily lost in our population of adenocarcinoma.But regarding the specific methylation studies, they are underway,and hopefully we will have the data for you soon.

Lastly, our goal is to standardize the process of calling somethingas high-grade dysplasia or low-grade dysplasia. We’renot trying to redefine the characteristics necessary for oneto be high-grade or low-grade dysplasia. We believe that ifwe were to use genetic alterations (in fact, a number of geneticalterations, I guess not necessarily the specific genes thatare altered), as demonstrated by the field effect that we haveseen, I think it would result in better characterization and,hence, more standardized treatment. In the case of high-gradedysplasia, most studies have shown that greater than 50% ofcases already have invasive carcinoma or intramucosal carcinomaat the time of diagnosis. So I think it’s essential thatwe standardize our analysis. And just to add one more thingto that, the study by Reid and colleagues showed that they hadone sample which had heavy inflammation, and they found, thepathologists and the panel of experts, that the calling rangedfrom no dysplasia with inflammation all the way to intramucosalcarcinoma on the same slide, and I think that makes a very strongpoint to some objective method that the pathologists could useas an adjunct to their visual observations.

DR SCOTT J. SWANSON (Boston, MA): I enjoyed your paper. I thinkit’s excellent work. I think I see where you’reheading, which is some sort of screening method for Barrett’s.My question would be, do you get enough tissue through a biopsyforceps from an endoscopy to be able to do this kind of analysis?

Thanks.

DR RAJA: Actually, our ultimate goal was to be able to utilizethis test in the setting of biopsy samples. Biopsy specimenstraditionally have several crypts, and based on our abilityto individually microdissect out these samples, they provideenough genetic material for us to perform these studies. Infact, we had to do several optimization and validation studiesbefore we proceeded with our analysis to show that we did notsee a phenomenon that has been reported in the literature—somethingcalled artifactual loss of heterozygosity, a loss of heterozygositythat is due to experimental methods. I think that the next stepfor our project would be to move on to biopsy specimens frompatients with varying levels of dysplasia and to see if a similarpattern of genetic alteration correlates well with their degreeof dysplasia.

References

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Abstract
Introduction
Material and methods
Results
Comment
Discussion
References

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