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Expression of Her-2/neu in Human Lung Cancer Cell Lines by Immunohistochemistry and Fluorescence in Situ Hybridization and its Relationship to in Vitro Cytotoxicity by Trastuzumab and Chemotherapeutic Agents¹

Lung Cancer Program, Departments of Medicine, Pathology, Preventative Medicine and Biostatistics, University of Colorado Cancer Center, University of Colorado Health Sciences Center, Denver CO 80262

	ABSTRACT

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Overexpression of the Her-2/neu oncogene and receptor protein was reported in 20% of breast cancers and was associated with a poor prognosis. Her-2/neu expression was a predictor for response to trastuzumab, a monoclonal antibody that recognizes the Her-2/neu cell surface receptor. Data regarding the expression of Her-2/neu in lung cancer are far more limited, and there is little information regarding the influence of Her-2/neu expression and response to trastuzumab alone or in combination with chemotherapeutic agents. In this report we evaluated Her-2/neu gene expression by fluorescence in situ hybridization (FISH) and the cell surface expression of the Her-2/neu receptor by immunohistochemistry using the HercepTest and by FACS analysis in 31 lung cancer cell lines with 5 breast cancer cell lines as controls. By FACS, we found Her-2/neu overexpression (mean fluorescence intensity >8) in 2 of the 22 non-small cell lung cancer (NSCLC) cell lines (9%), none of 11 small cell lung cancer (SCLC) cell lines, and 4 of 5 breast cancer cell lines. A positive HercepTest (2+ or 3+) was found in 6 of 19 NSCLC cell lines (26%, 2+; 5%, 3+), 1 of 3 SCLC cell lines (33%), and 4 of 5 breast cancer cell lines (80%). One of 6 NSCLC cell lines examined (17%) had gene amplification with >32 copies of Her-2/neu/cell and had homogeneous staining regions. One NSCLC cell line had a maximum of 14 copies of Her-2/neu/cell, and 3 had modest increases in Her-2/neu gene copy number without gene amplification (maximum 5–8 copies/cell). None of the SCLC cell lines had more than a maximum of 4 copies/cell, whereas the 2 breast cancer cell lines had maximum Her-2/neu copy numbers of 80 and 5, respectively. Aneusomy rather than true amplification was the major cause of increased Her-2/neu expression in most of the NSCLC cell lines. There was a strong correlation when the results of fluorescence-activated cell sorter, HercepTest results, and FISH were compared in pairs. Furthermore, Trastuzumab produced a G₁ cell cycle arrest and growth inhibition only in cell lines expressing Her-2/neu. The IC₅₀ for growth inhibition was correlated with cell surface Her-2/neu expression. The combination of trastuzumab and chemotherapeutic agents produced more than additive growth inhibition in cell lines expressing Her-2/neu, but the level of additivity was not related to the amount of Her-2/neu expression. These data indicate that trastuzumab alone and in combination with chemotherapeutic agents should be tested in NSCLC patients and that Her-2/neu should be assessed by both immunohistochemistry and FISH methods in these studies to determine which test is the best predictor of outcome.

	INTRODUCTION

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Lung cancer is the leading cause of cancer death in the United States and the world. In the United States it is the leading cause of cancer death in both males and females and kills more individuals than breast, colorectal, and prostate cancers combined (1) . The cure rate remains <15% despite some recent advances in chemotherapeutic agents (2) . Recent advances in biology and molecular biology have led to the development of targeted therapies. Overexpression of dominant oncogenes attributed to gene amplification, increased chromosome copy number, transcription, and other means have been reported to occur frequently in lung cancer, although these changes generally occur late in tumor development (3) . The erbB (Her) family of oncogenes is frequently overexpressed in lung cancer (4, 5, 6, 7, 8, 9, 10, 11, 12) . The erbB gene family encodes for growth factor tyrosine kinase receptors that are felt to play a role in the autocrine growth of human lung cancers (13, 14, 15, 16, 17) . The family consists of four receptors: erbB-1 (Her1), erbB-2 (Her-2/neu), erbB-3 (Her3), and erbB-4 (Her4). There are at least six ligands for these receptors. Binding of ligands to receptors causes heterodimerization and activation. In addition, Her-2/neu may be constitutively activated by mutation in cancer cells. The four receptors of this family are structurally similar with cysteine-rich domains, a membrane-spanning region, and an intracellular tyrosine kinase domain. Variable sequences in the cytoplasmic tail of each family member results in the recruitment and interaction of different second messengers and, thus, activation of downstream signal transduction pathways. Ligand binding to the extracellular domain initiates erbB receptor homo- and heterodimerization that expands the signaling diversity in this family of proteins. Signaling by receptor heterodimers may dominate over that of homodimers. Her2/neu has no known natural ligands and is the preferred heterodimeric partner for Her family ligand complexes.

Whereas the Her-2/neu proto-oncogene was originally identified as a dominant transforming oncogene produced as a result of point mutations, the gene (located on human chromosome 17) is frequently overexpressed by gene amplification rather than by mutation in human cancers (18, 19, 20) . The degree of overexpression/amplification correlates with poor prognosis and also with lack of response to conventional therapy (4, 5, 6, 7, 8, 9, 10, 11, 12 , 18, 19, 20, 21, 22) . Her-2/neu protein overexpression is most often measured by IHC using one of several monoclonal antibodies, and gene expression is measured most often by FISH³ for clinical studies. In a recent study in breast cancer, FISH provided superior prognostic information (23) . It is not known which test is the best predictor of response to targeted therapy.

The recognition of the role of the Her-2/neu signaling pathway in breast cancer led to the development of new treatment strategies designed to interfere with the pathway. One of the first approaches was to develop a monoclonal antibody to the Her-2/neu receptor that would block signal transduction and growth (24 , 25) . In preclinical models trastuzumab (Herceptin), a humanized monoclonal antibody, was shown to inhibit the growth of human breast cancers. This led to clinical trials where the antibody was shown to produce objective responses in a minority of Her-2/neu-positive patients (24) . In combination with doxorubicin- or paclitaxel-based therapy, trastuzumab produced higher response rates and longer survival than either agent alone (25) .

Studies of Her-2/neu in lung cancer have lagged behind those in breast cancer. Previous studies suggest that overexpression of Her-2/neu imparts a poor prognosis in NSCLC as it does in breast cancer and that overexpression occurs in about 20% of cases (4, 5, 6, 7, 8, 9, 10, 11, 12) . However, there is little information about the role of trastuzumab in the treatment of lung cancer. Thus, the goals of this study were to determine the degree and molecular mechanism of Her-2/neu overexpression in a panel of lung cancer cell lines. Additionally, we sought to determine the effect of trastuzumab alone and in combination with cytotoxic chemotherapy agents on the growth of human lung cancer cell lines in vitro.

	MATERIALS AND METHODS

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Cell Lines and Culture Conditions.
The NSCLC cell lines NCI-H322, NCI-H226, NCI-H441, NCI-H1703, NCI-H324, NCI-H2122, NCI-H125, NCI-H1334, NCI-H1435, NCI-H157, NCI-H1264, NCI-H661, NCI-H520, and NCI-H460 were kindly provided by Drs. John Minna and Adi Gazdar (University of Texas Southwestern Medical School, Dallas, TX). The SCLC cell lines NCI-H345, NCI-H209, NCI-H187, NCI-H69, NCI-H510, NCI-H146, NCI-H128, NCI-H82, NCI-H196, and NCI-N417 were also provided by Drs. John Minna and Adi Gazdar. The NSCLC line COLO699 was obtained from Dr. George Moore (Denver General, Denver, CO); the NSCLC line SW1573 was kindly provided by Dr. Hal Broxterman (Free University, Amsterdam, The Netherlands), and the NSCLC NE-18 was obtained from Dr. Karen Kelly (University of Colorado Health Science Center, Denver, CO). All of the above cell lines were maintained in RPMI 1640 (Life Technologies, Inc., Grand Island, NY) supplemented with 10% heat-inactivated FBS (Hyclone, Logan, UT) or in serum-free containing hydrocortisone, insulin, transferrin, estradiol, selenium (HITES) medium (26) . The SCLC cell line SHP-77 was kindly provided by Dr. Aurelio Koros (University of Pittsburgh, Pittsburgh, PA) and maintained in RPMI 1640 with 10% FBS. The NSCLC lines A549, Calu-3, SKLU-1, and the breast cancer cell line SKBR3 were obtained from the American Type Culture Collection, Rockville, MD, and were maintained in RPMI 1640 supplemented with 10% FBS or MEM supplemented with 0.1 mM nonessential amino acids, 1.0 mM sodium pyruvate, and 10% FBS. The breast cancer cell lines ZR75, MCF7, T747D. and MDA MB231were obtained from Dr. Kathryn Horwitz (Univ. of Colorado Cancer Center) and were maintained in RPMI 1640 media supplemented with 10% FBS. All of the cell lines were grown in 5% CO₂ at 37°C in incubators with 100% humidity.

Chemicals.
Trastuzumab was kindly provided by Genentech, Inc., South San Francisco, CA. The gemcitabine was provided by Eli Lilly, Indianapolis, IN. The paclitaxel was kindly provided by Bristol Myers-Squibb, Princeton, NJ. The cisplatin was purchased from Sigma Chemical Co. (St. Louis, MO). Glaxo-Wellcome, Research Triangle Park, NC, kindly provided the vinorelbine.

MTT Growth Assay.
Cell growth was assessed using a MTT assay (27) . Briefly, 10,000 viable cells were plated in 100-µl 96-well plates (Corning, Ithaca, NY). After an overnight incubation, various cytotoxic chemotherapy agents and/or trastuzumab were added in varying concentrations to each of three replicate wells and incubated for 6 days. After 6 days, the tetrazolium salt was added at a concentration of 0.4 mg/ml to each well. The microtiter plates were incubated with the salt for 4 h at 37°C and then the medium was aspirated off leaving the dark blue formazan product in the bottom of the wells. The reduced MTT product was solubilized by adding 100 µl of 0.2 N HCl in 75% isopropanol to each well. Thorough mixing was done using a Titertek multichannel pipetman (Flow Laboratories). The absorbency of each well was measured using an automated plate reader (Molecular Devices, Sunnyvale, CA). For each concentration the mean value ± the SE was calculated. When cell lines were incubated with combinations of trastuzumab and chemotherapeutic agents, the combination effects were assessed with the isobologram method of Chou and Talalay (28) .

Cell Cycle Distribution and Apoptosis.
The effects of trastuzumab on cell cycle distribution and percentage of apoptotic cells was determined by flow cytometric and immunofluorescence assays. At 72–120 h after incubation with trastuzumab, 1 x 10⁵ SHP-77, SKBR3, Calu-3, H157, and A549 cells were stained with 2.5% propidium iodide solution/0.3% saponin/0.001% RNase A in 10 mM EDTA. Stained nuclei were analyzed by using a Coulter EPICS XL-MCL (Coulter Corp., Miami, FL) for the proportions of cells in the G₀/G₁, S, and G₂-M phases of the cell cycle. Cell cycle studies were conducted twice as shown in the results. The resulting DNA distributions were analyzed using the Modfit LT Software (Verity House Software, Topsham, Maine; Ref. 29 ). The presence of apoptotic cells was confirmed by fluorescence microscopy.

Immunofluorescence Staining.
For FACS analysis, cells (5 x 10⁵) were incubated with the monoclonal antihuman HER-2/neu antibody c-erbB-2 Ab-2(9G6.10; NeoMarkers, Fremont, CA) or the isotype matched control mineral oil plasmacytoma-10 (Sigma Chemical Co.). The cells were counterstained with goat antimouse IgG1-FITC (Southern Bio-technology, Birmingham, AL). All of the staining was done on ice for 45 min followed by three washes in HBSS + 5% FBS. After staining, the cell fluorescence was measured by flow cytometry (Coulter EPICS-XL-MCL; Coulter Corp.). Using the Coulter software, the percentage of positive cells and their MFI were determined by comparison with the isotype matched control stained cells. For IHC analysis the cell lines were centrifuged into a cell pellet and embedded in paraffin for immunohistochemical staining with the HercepTest (Dako, Corp., Carpinteria, CA). Antigen retrieval was performed at 95°C in citrate buffer pH 6.0, 6.4 M sodium citrate dihydrate, 1.6 M citric acid monohydrate for 40 min. The slides were cooled at room temperature for 20 min and washed 3 x 3 min with Tris buffer pH 7.6, 0.15 M sodium chloride, 0.05 M Trizma HU. The slides were peroxidase block for 5 min and washed as above. The slides were incubated for 30 min with the primary antigen, followed by the secondary antigen (Visualization Reagent), followed by the substrate-chromogen solution (3,3'-diaminobenzidine), and finally counter stained with hematoxylin. The breast cancer cell SKBR3 known to be positive for HER-2/neu overexpression was used as a positive control. For a negative control, the primary antibody was replaced by a nonspecific negative control antibody. References pathologists (W. R. F., F. R. H.) quantified membrane staining as 0–3+ according to the Dako instructions. Each pathologist independently scored the samples. The few discrepancies were resolved by joint review of samples with discrepant results.

FISH.
Cell suspensions were dropped onto a microscope slide and incubated for 30 min at 37°C in 2 x SSC followed by ethanol dehydration, a 30-s wash in 70% acetic acid, and ethanol dehydration. The PathVysion HER-2/neu DNA probe kit (Locus Specific Indicator LSI) Her-2/neu labeled in SpectrumOrange)/chromosome enumerator probe (CEP) chromosome 17 labeled in SpectrumGreen from Vysis (Dowers Grove, IL) was applied to the slides according to the manufacturer’s directions, and the slides were incubated for 10 min at 80°C for codenaturation of probe and chromosomal DNA. Hybridization proceeded overnight at 37°C. After hybridization, the slides were washed in 50% formamide/2 x SCC/0.1% NP40 at 46°C. The chromatin was counterstained with 4',6-diamidino-2-phenylindole in Vectashield antifad (Vector, Burlingame, CA). A minimum of 200 nuclei were scored under a BX60 Olympus fluorescence microscope (Olympus, Boston, MA), using a triple band pass interference filter (blue/red/green) and a single band filter for blue, red, and green. Images were acquired using a cooled CCD camera (SenSys; Photometrics, Tucson, AZ) and merged using the SmartCapture software from Vysis.

Statistical Comparisons.
Comparisons between the Her-2/neu protein expression as assessed by MFI in NSCLC versus SCLC, NSCLC versus breast cancer, and SCLC versus breast cancer cell lines were done using a Wilcoxon rank-sum test. Comparisons of the fraction of cells in the cell cycle distributions were performed using a ² test. Correlation coefficients for comparisons of maximum Her-2/neu gene versus average Her-2/neu gene expression, Max Her-2/neu gene expression versus MFI, and IHC versus MFI were calculated as the Spearman correlation coefficient.

	RESULTS

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Her-2/neu Expression.
The cell surface expression of Her-2/neu as assessed by FACS and IHC HercepTest is shown in Figs. 1 and 2 and summarized in Table 1B . By FACS analysis, 3 of 22 NSCLC cell lines (14%) had no cells expressing Her-2/neu. Twelve NSCLC cell lines (55%) had low Her-2/neu protein levels with a MFI of <4, 5 NSCLC lines (23%) had moderate expression (MFI between 4 and 8), and 2 NSCLC lines (9%) had high expression with a MFI >8. Only 1 of 11 SCLC cell lines (9%) expressed any Her-2/neu with a low MFI of 3.7. Four of 5 breast cancer cell lines (80%) expressed high levels of Her-2/neu with a MFI >8 (Fig. 1A) . Among the lung cancer cell lines of various histology, the adenocarcinomas had the highest expression with an average MFI of 6.8 (range 0–36; median 3.8). The large cell carcinomas had an average MFI of 3.4 (range 2.4–4.7; median 3), and squamous carcinomas had an average MFI of 3.1 (range 0–4.3; median 3). SCLC cell lines had the lowest expression with only 1 cell line showing any expression (average MFI of 0.34). Breast cancer cell lines had an average MFI of 16. The differences in Her-2/neu expression between breast cancer and both NSCLC and SCLC cell lines were statistical significant (Wilcoxon rank-sum test; P < 0.001). The differences between the NSCLC cell types were not different. The NSCLC cell lines had significantly greater expression than the SCLC cell lines (P = 0.0002).

View larger version (32K): [in this window] [in a new window] [Download PPT slide]   Fig. 1. Expression of Her-2/neu in four representative cells lines as assessed by FACS analysis using the 9G6.10 antibody. A, expression of Her-2/neu in the breast cancer cell line SKBR3. Compared with SKBR3 cells stained with the irrelevant antibody shown in the left peak, >99% of the SKBR3 cells were positive, and the MFI was 43 units. This was scored as 3+ positivity because the MFI exceeded 8 units. B, Her-2/neu expression in the NSCLC cell line Calu3 stained with the irrelevant antibody, left peak, and with the 9G6.10 antibody, right peak. Cells (>99%) were positively stained with a MFI of 36 units. C, expression of the NCI-H322 cells stained with the irrelevant antibody or 9G6.10. Positive staining was present in >98% of the cells with a MFI of 9.8. D, FACS analysis of the NSCLC cell line A549 with 72% of the cells stained positively with a MFI of 3.7 units (1+).

View larger version (126K): [in this window] [in a new window] [Download PPT slide]   Fig. 2. Expression of Her-2/neu in four cell lines as assessed by IHC. A, 1+ expression in NSCLC cell line H2122. B, 2+ Her-2/neu staining of the NSCLC cell line H661. C, 3+ Her-2/neu staining of the NSCLC Calu-3 cell line. D, 3+ Her-2/neu staining of the breast cancer cell line SKBR3.

The results comparing IHC to FACS are shown in Fig. 3A . There was an excellent correlation (r = 0.57; P = 0.002) between Her-2/neu cell surface expression assessed by IHC or FACS. Using criteria of 0 or 1+ HercepTest and MFI 4 as negative and 2+ or 3+ HercepTest and MFI >6 as positive, 15 cell lines had no expression by either test, and 7 cell lines were positive by both methods. Five lung cancer cell lines had discordant results: a 2+/3+ HercepTest and negative MFI <4 in 3 cell lines and HercepTest 0/1+ with an MFI of 4–8 in 2 cell lines.

View larger version (26K): [in this window] [in a new window] [Download PPT slide]   Fig. 3. Correlation of various assessments of Her-2/neu cell surface expression by various methods and Her-2/neu gene copy number by histology , Adeno; , Squamous; , Large; , SCLC; , Breast. A, correlation between the cell surface Her-2/neu expression as assessed by IHC and by FACS with 27 cell lines that had both tests performed. There was an excellent correlation (r = 0.57; P = 0.002). The correlation was best at the highest and lowest values. B, correlation between the average and maximum number of copies of the Her-2/neu gene/cell. The correlation was excellent across all histologies (r = 0.91; P = 0.0003). C, correlation between the cell surface expression by FACS (MFI) and the maximum gene copy number as assessed by FISH in the 10 representative cell lines that had both analyses done. Once again, there was an excellent correlation (r = 0.76; P = 0.011). D, maximum copies of Her-2/neu gene by histology.

View larger version (65K): [in this window] [in a new window] [Download PPT slide]   Fig. 4. Her-2/neu gene status determined in FISH assays using the Her-2 PathVysion DNA probe. Gene amplification was detected in the breast cancer cell line SKBR3 (A) and in the lung adenocarcinoma cell line Calu-3 (B). Metaphase analysis revealed that the gene amplification in Calu-3 was represented by hsrs located in two derivative chromosomes (C). These chromosomes were identified by Spectral Karyotyping technique as derivatives of t(2;17) and t(12;17; 4D). A third derivative [der(17)t(15;16;17)] carried an apparently normal copy of the gene. The NCI-H322 lung adenocarcinoma cell line showed unbalanced aneusomy with higher number of copies per cell of the Her-2/neu gene than of chromosome 17 (E), whereas the lung adenocarcinoma A549 cell line exhibited balanced aneusomy with similar increase in gene and chromosome numbers per cell (F).

Three of 6 NSCLC cell lines examined by FISH had maximum Her-2/neu gene copy numbers of five to eight with average copy numbers of three to four and chromosome 17 numbers of three to 5.3. For example, the A549 adenocarcinoma (Fig. 4F) and the NCI-H460 (data not shown) large cell carcinoma cell lines had weak cell surface protein expression (MFI, 3.7 and 2.4, respectively) and showed balanced aneusomy by FISH. The A549 line was near triploid with an average of 3.7 copies of both chromosome 17 and the Her-2/neu gene/cell. NCI-H460 was hyperdiploid with trisomy for both chromosome 17 and Her-2/neu, whereas 1 of 200 cells had a clustered gene amplification. Unbalanced aneusomy was observed in some NSCLC lines. For example, the NCI-H1435 line had an average of 5.3 copies of chromosome 17/cell but only three copies of Her-2/neu (data not shown). The centromeric signal was found in four distinct types of chromosome, none of which resembled a normal chromosome 17. Other chromosomes carrying chromosome 17 material were a large metacentric and a medium-sized submetacentric chromosome detected in 50% of the cells with one copy/cell. The most common was a small acrocentric chromosome probably del(17)(q11) usually present in more than two copies/cell. A large metacentric and a medium-sized submetacentric chromosome were detected in 50% of the cells with one copy/cell. These three chromosomes carried no Her-2/neu sequences. The other derivative 17 was medium sized and metacentric with Her-2/neu sequences close to the centromere. In addition, two copies of a large submetacentric chromosome, der(14)t(8;6;14;17), also carried the Her-2/neu sequences in the distal region of the short arm. Although the ratio of Her-2/neu:chromosome 17 was <1, the gene copy number per cell matched the ploidy level of 3n, and the protein expression observed may have been attributable to the aneusomy. One NSCLC cell line had a maximum and average Her-2/neu copy number of two per cell.

SCLC cell lines never had Her-2/neu gene amplification, and both cell lines examined had balanced aneusomy. For example, the NCI-H345 cell line was near triploid with an average of three copies of chromosome 17 per cell, each harboring one copy of Her-2/neu (data not shown). In the near diploid SHP-77, there were three copies of normal or derivative chromosome 17 per cell but only two copies of Her-2/neu, because one derivative was an isochromosome of the short arm (data not shown). The fact that no cell surface Her-2/neu expression was observed in these SCLC cell lines indicates that there are also abnormalities in gene transcription or translation or post-translational modification of the protein in SCLC cells.

There was an excellent correlation (r = 0.91; P = 0.0003) between the maximum and average Her-2/neu gene copy number per cell (Fig. 3B) . There was also an excellent correlation (r = 0.76; P = 0.011) between the maximum gene copy number and the MFI cell surface expression (Fig. 3C) . Both cell lines (SKBR3 and Calu-3) with marked gene amplification and copy numbers exceeding 32 had marked Her-2/neu protein overexpression with MFIs of 43 and 36, respectively, and 3+ HercepTest. One NSCLC cell line (NCI-H322) had a maximum gene copy number of 14 and an MFI of 9.8 with a 2+ HercepTest. Weak cell surface expression (MFI 4 and HercepTest 0 or 1+) was observed in 7 lung cancer cell lines that all had maximum Her-2/neu gene copy numbers of less than eight. By cell type, the average maximum Her-2/neu gene copy number per cell was 23 for adenocarcinoma, 6 for large cell carcinoma, 4 for small cell carcinoma, 2 for squamous carcinoma, and 42 for breast cancer cell lines (Fig. 3D) .

Effects of Trastuzumab on Cell Cycle Distribution.
The effects of trastuzumab on the cell cycle distribution in the breast cancer cell line SKBR3; the NSCLC cell lines Calu-3, NCI-H322, A549, and NCI-H157; and the SCLC cell line SHP-77 are shown in Table 2 . In the SKBR3 breast cancer cells, trastuzumab produced a statistically significant G₁ cell cycle arrest with the percentage of cells in G₁ increasing from 63% to 68% with a corresponding decrease in the fraction of cells in S phase from 25% to 20%. Trastuzumab also produced a G₁ cell cycle arrest in the Her-2/neu-expressing NSCLC cell lines Calu-3 (MFI 36) and NCI-H322 (MFI 9.8) with an increase in G₁ from 41% to 47% and 57% to 62% in the two lines, respectively. In the low expressing NSCLC line A549 (MFI 3.7), there was a smaller increase in the G₁ fraction from 69% to 71%. There was no change in the cell cycle distribution in NCI-H157, which has low HER-2/neu expression (MFI 2.8) and SHP-77 cells, which lack Her-2/neu cell surface protein expression. No apoptosis was seen in any cell line after a 120-h exposure to trastuzumab.

View larger version (18K): [in this window] [in a new window] [Download PPT slide]   Fig. 5. Effects of trastuzumab on the growth of breast and NSCLC cells in MTT assays. Trastuzumab inhibit the growth of the breast cancer cell line SKBR3 () in a dose-dependent fashion with inhibition noted at concentrations as low as 1 µM. SE bars show the variability in results. Trastuzumab produced no inhibition of Her-2/neu negative cell lines at any concentration (e.g., the SCLC cell line SHP-77 ). Trastuzumab produced some growth inhibition of the Her-2/neu expressing NSCLC cell lines A549 () and NCI-H322 () but only at higher concentrations than SKBR3.

View larger version (61K): [in this window] [in a new window] [Download PPT slide]   Fig. 6. CI values for the combination of trastuzumab with gemcitabine in four cell lines including the 3+ breast cancer cell line SKBR3 (A), the 2+ NSCLC cell line NCI-H322 (B), the 1+ NSCLC cell line A549 (C), and the nonexpressing SCLC cell line SHP-77 (D). Synergistic growth inhibitory effects were observed in the three Her-2/neu-expressing lines, but antagonistic effects were noted in the nonexpressing SHP-77 cells.

	DISCUSSION

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The results of this study show that NSCLC cell lines often express moderate levels of cell surface Her-2/neu, whereas SCLC cell lines do not. The level of expression of cell surface Her-2/neu in the NSCLC cell lines is lower than in breast cancer cell lines, and the mechanism of overexpression is different. Whereas breast cancer cell lines overexpress Her-2/neu because of gene amplification in the majority of cases (17 , 18) , we found that gene amplification occurred infrequently in NSCLC cell lines (17%). Only the Calu-3 cell line had true gene amplification with a Her-2/neu gene:chromosome 17 ratio exceeding 2. One additional NSCLC cell line had a maximum Her-2/neu gene copy number of 14 with an average of 6.5. We found that the low to moderate cell surface expression of Her-2/neu in NSCLC is most often attributable to increased copy number from chromosome duplication and polysomy. For example, the cell line NCI-H322 has 6.5 copies of Her-2/neu and 5.7 copies of chromosome 17, and A549 has 3.7 copies of the gene and chromosome. In other studies the frequency and degree of Her-2/neu cell surface expression in lung cancer specimens (defined as 2+ or 3+) ranged from 13% to 54% and averaged 31% (2, 3, 4, 5, 6, 7, 8, 9, 10, 11, 12) . In this study, 26% (5/19) of NSCLC cell lines were 2+ or 3+ by HercepTest, but only one was 3+. By FACS analysis 32% (7/22) had a MFI >4, but only 2 (9%) had an MFI >8. Total absence of Her-2/neu expression was uncommon in NSCLC cell lines, because only 3 had no cell surface expression by FACS, only 1 had a maximum gene copy number <4, and 7 had 0+ staining by HercepTest. The majority of NSCLC cell lines had mild to moderate Her-2/neu expression, 16 by all three methods including 77% by FACS, 67% by FISH, and 58% by HercepTest.

This communication is the first report with detailed comparisons of Her-2/neu expression by FACS, IHC, and FISH in lung cancer cell lines. There are several ways to quantitate Her-2/neu gene expression by FISH including the average or maximum copy number, the ratio of copy number:chromosome number, or the percentage of cells with unbalanced copy number. We found a good correlation of the results of each of these analyses in this study and in a study of samples from lung cancer patients (20) . Among the 53 lung cancer patient samples evaluated by FISH in the companion study, we found few instances of gene amplification (5%) and many instances of increased copy number (20%) among 45 NSCLC patient tumors. There were no instances of gene amplification or copy number >4 in SCLC tumors, and no SCLC specimen had >1+ protein expression. In the present study of lung cancer cell lines and in breast cancer series in the literature, there was a good correlation between the FISH method of assessing Her-2/neu gene status and either the FACS or IHC method of assessing cell surface protein expression.

In literature studies of NSCLC, Her-2/neu expression has been assessed predominantly by IHC. The majority of studies found a direct relationship between prognosis and Her-2/neu expression with shorter survival in Her-2/neu+ cases. In some reports, patients of which their tumors expressed Her-2/neu were less likely to respond to chemotherapy (22) . In breast cancer, recent reports suggest that gene amplification is a superior method for assessing prognosis than protein expression by IHC (23) . It needs to be determined whether increased copy number without amplification will be associated with a poor prognosis in NSCLC and whether FISH results will provide superior prognostic information compared with IHC.

There is little information in the literature regarding Her-2/neu gene or protein expression in NSCLC cells and the likelihood of response to trastuzumab alone or with chemotherapy. Both gene amplification and cell surface expression have been reported to predict response to trastuzumab alone or combined with doxorubicin or paclitaxel in breast cancer (19 , 24) . Recent evidence shows that gene amplification by FISH is the best predictor of response, and patients without gene amplification appear to have little benefit from trastuzumab therapy. This would imply that only a small fraction of NSCLC patients and no SCLC patients would benefit from trastuzumab therapy (19) . Despite the fact that Her-2/neu overexpression and gene amplification occur less frequently in NSCLC than breast cancer, we found that marked synergistic growth inhibition occurred when standard cytotoxic chemotherapy was combined with trastuzumab in Her-2/neu-expressing NSCLC cell lines. We found a direct relationship between Her-2/neu expression and both cell cycle arrest and growth inhibition, but the synergy with chemotherapy was independent of the degree of expression in cell lines that expressed any level of cell surface Her-2/neu expression. Trastuzumab had no effect on cell cycle distribution, growth rate, or synergy with chemotherapy in nonexpressing cell lines. The results of this study predict that trastuzumab alone will produce partial objective responses in some NSCLC patients of which their tumors express Her-2/neu. Furthermore, the best responses will occur in the uncommon patient with marked HER-2/neu overexpression by gene amplification, because only Her-2/neu-expressing cell lines were growth inhibited, and the high expressing Calu-3 line was growth inhibited the most. The study results also suggest that synergy between trastuzumab and chemotherapeutic agents will exist in lung cancer as it does in breast cancer if the tumor expresses Her-2/neu, even if the degree of expression is low. Additionally, the results of this study suggest that among all of the agents tested here, the greatest synergy may exist between trastuzumab and gemcitabine. On the basis of this study, patients with overexpression of Her-2/neu should be considered for clinical trials. Randomized Phase III trials of chemotherapy alone versus chemotherapy plus trastuzumab in NSCLC patients with gene amplification would be most likely to determine the role for trastuzumab in NSCLC, but these studies will require intergroup participation because of the low frequency of gene amplification.

A number of clinical trials have been instituted in the first and second line therapy of advanced lung cancer. There are no randomized trials evaluating trastuzumab in NSCLC patients, but preliminary results from Phase II combination studies are just appearing in the literature (30) . Randomized trials will be warranted if the response rates do not appear higher than those in historical series; the number of patients with 3+ Her-2/neu expression or gene amplification is very small, and these 3+ patients appear to do worse when treated with chemotherapy alone.

	FOOTNOTES

 
The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore be hereby marked advertisement in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

¹ Supported by National Cancer Institute Grants CA 46934-09 and CA 58187-04.

² To whom requests for reprints should be addressed, at University of Colorado Cancer Center, Box B188, 4200 East Ninth Avenue, Denver, CO 80262.

³ The abbreviations used are: FISH, fluorescence in situ hybridization; SCLC, small cell lung cancer; NSCLC, non-small cell lung cancer; hsr, homogeneously staining region; MFI, mean fluorescence intensity; MTT, 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide; FBS, 10% heat inactivated fetal bovine serum; FACS, fluorescence-activated cell sorting; IHC, immunohistochemistry; CI, combination index.

Received 2/15/01; revised 6/22/01; accepted 6/25/01.

	REFERENCES

Top ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

 

1. Greenlee R. T., Murray T., Bolden S., Wingo P. A. Cancer statistics 2000. CA Cancer J. Clin., 50: 7-33, 2000.[Abstract]
2. Bunn P. A., Kelly K. New chemotherapeutic agents prolong survival and improve quality of life in non-small cell lung cancer: a review of the literature and future directions. Clin. Cancer Res., 5: 1087-1100, 1998.
3. Kelly M. T., Johnson B. E. Genetic mechanisms of solid tumor oncogenesis. Adv. Intern. Med., 39: 93-122, 1994.[Medline]
4. Harpole D. H., Jr., Marks J. R., Richards W. G., Herndon J. E., II, Sugarbaker D. L. Localized adenocarcinoma of the lung: oncogene expression of erbB-2 and p53 in 150 patients. Clin. Cancer Res., 1: 659-664, 1995.[Abstract]
5. Kern J. A., Schwartz D. A., Nordberg J. E., Weiner D. B., Greene M. I., Torney K., Robinson R. A. p185neu expression in human lung carcinomas predicts shortened survival. Cancer Res., 50: 5184-5191, 1990.[Abstract/Free Full Text]
6. Schneider P. M., Praeuer H. W., Sroeltzing O., Boehm J., Manning J., Metzer R., Fink U., Wegerer S., Hoelscher A. H., Roth J. A. Multiple molecular marker testing (p53, c-Ki-ras, c-erbB-2) improves estimation of prognosis in potentially curable resected non-small cell lung cancer. Br. J. Cancer, 83: 473-479, 2000.[CrossRef][Medline]
7. Scheurle D., Jahanzeb M., Aronsohn R. S., Watzek L., Narayanan R. HER-2/neu expression in archival non-small cell lung carcinoma using FDA-approved Hercep test. Anticancer Res., 20: 2091-2096, 2000.[Medline]
8. Langer C., Adak S., Thor A., Johnson D. Phase II Eastern Cooperative Oncology Group (ECOG) pilot study of paclitaxel, carboplatin and trastuzmab in HER2/neu + advanced NSCLC: preliminary analysis. Lung Cancer, 29 (Suppl. 2): 142 2000.
9. Tateishi M., Ishida T., Mitsudomi T., Kaneko S., Sugimacline K. Prognostic value of c-erbB-2 protein expression in human lung adenocarcinoma and squamous cell carcinoma. Eur. J. Cancer, 27: 1372-1375, 1991.
10. Hsieh C. C., Chow K. C., Fahn H. J., Tsai C. M., Li W. Y., Huang M. H., Wang L. S. Prognostic significance of HER-2/neu overexpression in stage I adenocarcinoma of the lung. Ann. Thorac. Surg., 66: 1159-1163, 1998.[Abstract/Free Full Text]
11. Yu D., Wang S. S., Dulski K. M. c-erbB-2/neu overexpression enhances metastatic potential of human lung cancer cells by induction of metastasis-associated properties. Cancer Res., 54: 3260-3266, 1994.[Abstract/Free Full Text]
12. Kern J. A., Slebos R. J., Top B., Rodenhuis S., Lager D., Robinson R. A., Weiner D., Schwartz D. A. c-erb-2 expression and codon 12 K-ras mutations both predict shortened survival for patients with pulmonary adenocarcinomas. J. Clin. Investig., 93: 516-520, 1994.
13. Klapper L. N., Kirschbaum M. H., Sela M., Yarden Y. Biochemical and clinical implications of the ErbB/HER signaling network of growth factor receptors. Adv. Cancer Res., 77: 25-79, 2000.[Medline]
14. Beerli R. R., Hynes N. E. Epidermal growth factor-related peptides activate distinct subsets of ErbB receptors and differ in their biological activities. J. Biol. Chem., 271: 6071-6076, 1996.[Abstract/Free Full Text]
15. Graus-Porta D., Beerli R. R., Daly J. M., Hayner N. E. ErbB-2, the preferred heterodimerization partner of all ErbB receptors, is a mediator of lateral signaling. EMBO J., 16: 1647-1655, 1997.[CrossRef][Medline]
16. Pinkas-Kramarski R., Shelly M., Guarino B. C., Wang L. M., Lyass L., Alroy I., Alimandi M., Kuo A., Moyer J. D., Lavi S., Eisenstein M., Ratzkin B. J., Serger R., Bacus S. S., Pierce J. H., Andrews G. C., Yarden Y. ErbB tyrosine kinases and the two neuregulin families constitute a ligand receptor network. Mol. Cell Biol., 18: 6090-6101, 1998.[Abstract/Free Full Text]
17. Lonardo F., DiMarco E., King C. R., Pierce J. H., Segatto O., Aaronson S. A., DiFiore P. P. The normal erbB-2 product is an atypical receptor-like tyrosine kinase with constitutive activity in the absence of ligand. New Biol., 2: 992-1003, 1990.[Medline]
18. Harbeck N., Ross J. S., Yurdseven S., Dettmar P., Polcher M., Kuhn W., Ulm K., Graeff H., Schmitt M. HER2 gene amplification by fluorescence in situ hybridization allows risk group assessment in node negative breast cancer. Int. J. Oncol., 14: 663-671, 1999.[Medline]
19. Mass R. D., Sanders C., Charlene K., Johnson L., Everett T., Anderson S. The concordance between the clinical trials assays (CTA) and fluorescence in situ hybridization (FISH) in the herceptin pivotal trials. Proc. Am. Soc. Clin. Oncol., 19: 75a 2000.
20. Hirsch F., Veve R., Varella-Garcia L., Bunn P. A., Franklin W. Evaluation of HER2/neu expression in lung cancer tumors by immunohistochemistry and fluorescence in situ hybridization. Lung Cancer, 29 (Suppl. 1): 211 2000.
21. Slamon D., Godolphin W., Jones L. A., Holt J. A., Wong S. G., Keith D. E., Levin W. J., Stuart C. G., Udove J., Ullrich A. Studies of the HER-2/neu proto-oncogene in human breast and ovarian cancers. Science (Wash. DC), 244: 707-712, 1989.[Abstract/Free Full Text]
22. Tsai C. M., Chang K. T., Perng R. P., Mitsudomi T., Chen M. H., Kadoyama C., Gadzar A. F. Correlation of intrinsic chemoresistance of non-small cell lung cancer cell lines with HER2/neu gene expression but not with ras gene mutations. J. Natl. Cancer Inst., 85: 897-901, 1993.[Abstract/Free Full Text]
23. Pauletti G., Dandekar S., Rong H. M., Ramos L., Peng H., Seshadri R., Slamon D. J. Assessment of methods for tissue-based detection of the Her-2/neu alteration in human breast cancer: a direct comparison of fluorescence in situ hybridization and immunohistochemistry. J. Clin. Oncol., 18: 3651-3664, 2000.[Abstract/Free Full Text]
24. Slamon D. J., Leyland-Jones B., Shak S., Paton V., Bajamonde A., Fleming T., Eiermann W., Woler J., Barelga J., Norton L. Addition of herceptin (humanized anti-HER-2 antibody) to first line chemotherapy for HER-2 overexpressing metastatic breast cancer markedly increases anti-cancer activity. Proc. Am. Soc. Clin. Oncol., 17: 98a 1998.
25. Baselga J., Norton L., Albanell J., Kim Y. M., Mendelson J. Recombinant anti-HER2 antibody (herceptin) enhances the antitumor activity of paclitaxel and doxorubicin against HER2/neu overexpressing human breast cancer xenografts. Cancer Res., 58: 2825-2831, 1998.[Abstract/Free Full Text]
26. Carney D. N., Bunn P. A., Jr., Gazdar A. F., Pagan J. A., Minna J. D. Selective growth in serum-free hormone-supplemented medium of tumor cells obtained by biopsy from patients with small cell carcinoma of the lung. Proc. Natl. Acad. Sci. (USA), 78: 3185-3189, 1981.[Abstract/Free Full Text]
27. Carmichael J., Mitchell J. B., DeGraff W. G., Gamson J., Gazdar A. F., Johnson B. E., Glatstein E., Minna J. D. Chemosensitivity testing of human lung cancer cell lines using the MTT assay. Br. J. Cancer, 57: 540-547, 1988.[Medline]
28. Chou T. C., Talalay P. Analysis of combined drug effects: a new look at a very old problem. Trends Pharmacol. Sci., 4: 450-454, 1983.
29. Yamamura Y., Rodriguez N., Schwartz A., Eylar E., Bagwell B., Yano N. A new flow cytometric method for quantitative assessment of lymphocyte mitogenic potentials. Cell. Mol. Biol., 41 (Suppl. 1): S121-S132, 1995.
30. Krug L. M., Miller V. A., Crapanzano J. P., Zakowski M. F., Heelan R. T., Ross J., Sheehan C., Venkatraman E., Pizzo B. A., McClean N. A., Kris M. G. Randomized phase II trial comparing trastuzumab plus weekly docetaxel versus trastuzmab plus weekly paclitaxel in previously untreated advanced non-small cell lung cancer. Lung Cancer, 29 (Suppl. 1): 57 2000.[Medline]

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