Prognostic impact of serum CYFRA 21-1 in patients with advanced lung adenocarcinoma: a retrospective study.

BACKGROUND: Serum CYFRA 21-1 is one of the most important serum markers in the diagnosis of non-small cell lung cancer (NSCLC), especially squamous-cell carcinoma. However, it remains unknown whether pretreatment serum CYFRA 21-1 values (PCV) may also have prognostic implications in patients with advanced lung adenocarcinoma.
METHODS: We retrospectively reviewed the data of 284 patients (pts) who were diagnosed as having advanced lung adenocarcinoma and had received initial therapy.
RESULTS: Of the study subjects, 121 pts (43%) had activating epidermal growth factor receptor (EGFR) mutations (Mt+), while the remaining 163 pts (57%) had wild-type EGFR (Mt-). Univariate analysis identified gender (male/ female), ECOG performance status (PS) (0-1/ ≥2), PCV (<2.2 ng/ml/ ≥2.2 ng/ml), EGFR mutation status (Mt+/ Mt-), pretreatment serum CEA values (<5.0 ng/ml/ ≥5.0 ng/ml), smoking history (yes/ no) and EGFR-TKI treatment (yes/ no) as prognostic factors (p = .008, p < .0001, p < .0001, p < .0001, p = .036, p = .0012, p < .0001 respectively). Cox's multivariate regression analysis identified PCV < 2.2ng/ml as the only factor significantly associated with prolonged survival (p < .0001, hazard ratio: 0.43, 95% CI 0.31-0.59), after adjustments for PS (p < .0001), EGFR mutation status (p = .0069), date of start of initial therapy (p = .07), gender (p = .75), serum CEA level (p = .63), smoking history (p = .39) and EGFR-TKI treatment (p = .20). Furthermore, pts with Mt+ and PCV of <2.2 ng/ml had a more favorable prognosis than those with Mt+ and PCV of ≥2.2 ng/ml (MST: 67.0 vs. 21.0 months, p < .0001), and patients with Mt- and PCV of <2.2 ng/ml had a more favorable prognosis than those with Mt- and PCV of ≥2.2 ng/ml (MST: 24.1 vs. 10.2 months, p < .0001).
CONCLUSION: PCV may be a potential independent prognostic factor in both Mt+ and Mt- patients with advanced lung adenocarcinoma.

Background

Lung cancer is the leading cause of cancer death, and at present, there exists no cure of stage IV non-small cell lung cancer (NSCLC) [1]. Adenocarcinoma and squamous cell carcinoma are the most common histological subtypes of lung cancer and account for about 70% of all lung cancers [2]. The folate antagonist pemetrexed has been shown to exhibit efficacy against non-squamous cell lung cancers [3], and is currently used in combination with cisplatin as a standard treatment regimen for patients with non-squamous cell lung carcinoma. Chemotherapy with the angiogenesis inhibitor bevacizumab administered in combination with platinum agents has also been shown to exhibit favorable efficacy against non-squamous cell lung carcinoma [4,5]. Somatic gain-of-function mutations in exons encoding the EGFR tyrosine kinase domain have been identified in NSCLC [6,7]. Several previous studies have reported prolongation of the survival time in patients with EGFR-mutation-positive lung carcinomas treated with EGFR-tyrosine kinase inhibitors (TKIs) [8-11], therefore, EGFR-TKIs are widely used in medical practice. EGFR mutations occur more frequently in lung cancer patients who are Asians, females and non-smokers with the histological subtype of adenocarcinoma [12-14]. On the other hand, while there have also been scattered reports of EGFR mutations among cases of lung squamous-cell carcinoma [15-17], a recent report showed that there were no EGFR mutation-positive cases among lung cancer patients with pure squamous cell carcinoma [18,19].

CYFRA 21–1 is a fragment of cytokeratin (CK) 19. CKs, which are now called keratins, are the principal structural elements of the cytoskeleton (keratin filaments) of epithelial cells, including bronchial epithelial cells, and have been classified into 20 subtypes based on differences in the molecular mass and isoelectric point as determined by 2-dimensional electrophoresis [20,21]. CK types 1–8 are categorized as type I CKs, and CKs 9–20 as type II CKs. Microfilaments are heteropolymers formed from type I and type II keratins, and constitute the cytoskeleton [22]. CK19 is a soluble type I CK (acidic type), and has the lowest molecular mass (40 kDa) among the CKs. It is expressed in the unstratified or pseudostratified epithelium lining the bronchial tree [23], and been reported to be overexpressed in many lung cancer tissue specimens [24]. The CK expression patterns in tissues are well-maintained even during the process of transformation of the tissue from normal to tumor tissue [25]. Accelerated CK19 degradation occurs in neoplastically transformed epithelial cells as a result of increased protease activity of caspase 3, a regulator of the apoptosis cascade, and fragments are released into the blood. This results in an increase of the blood CYFRA 21–1 values, because CK19 fragments are recognized by two monoclonal antibodies [26].

Measurement of serum CYFRA 21–1 level is a useful auxiliary test in the diagnosis of NSCLC, and particularly high specificity of this test has been reported for the diagnosis of squamous cell carcinoma of the lung [27,28]. On the other hand, a meta-analysis also revealed that serum CYFRA 21–1 may be a useful prognostic factor in NSCLC patients [29]; analysis of the histological background in the aforementioned meta-analysis showed that non-adenocarcinoma accounted for the majority of cases of NSCLC (65%). There has also been a report suggesting that serum CYFRA 21–1 levels might serve as a prognostic factor in patients with recurrent NSCLC receiving 3rd-line or later gefitinib therapy [30]. Some studies have suggested the possible prognostic value of pretreatment serum CYFRA 21–1 values (PCV) in patients with surgically treated lung adenocarcinoma [31] and advanced NSCLC [32-34]. However, none of the studies suggesting serum CYFRA 21–1 as a prognostic factor in patients with untreated advanced lung adenocarcinoma has included the EGFR mutation status as a variable. Therefore, in the present study, we investigated the impact of serum CYFRA 21–1 on the prognosis of untreated advanced lung adenocarcinoma patients.

Methods

Patients

Of patients diagnosed as having primary lung carcinoma between January 2003 and June 2010 at the Shizuoka Cancer Center, EGFR mutation analysis was performed on 424 patients from April 2008 to June 2010. Of these, 284 lung adenocarcinoma patients had received initial therapy, and we retrospectively reviewed the data of the 163 patients who were found to harbor wild-type EGFR and 121 patients who were found to harbor activating EGFR mutations (Figure 1). The following inclusion criteria were set for this study; patients with pathologically proven adenocarcinoma who had received initial therapy (including chemotherapy or chemoradiotherapy) and survived for more than one month; Eastern Cooperative Oncology Group performance status (ECOG PS) of 3 or less. The histological and cytological diagnoses were performed according to the WHO classification criteria [35]. The study was conducted with the approval of the Shizuoka cancer center Institutional Review Board #1 (HHS IRB registration number; IRB00006744).

Figure 1

A flow-diagram of the patients included in the analysis.

We outsourced some of the clinical laboratory tests, such as measurement of the tumor markers and EGFR mutation analysis. Serum CYFRA 21–1 and serum CEA concentrations were measured at the baseline, before the initial therapy. The serum CYFRA 21–1 concentration was measured using a Lumipulse Presto® kit (FUJIREBIO Inc, Tokyo, Japan), based on a CLEIA (chemiluminescent enzyme immunoassay) method, while the serum CEA concentrations were measured using an ARCHITECT® kit (Abbott Japan, Tokyo, Japan). EGFR mutation analysis was performed by fragment analysis using polymerase chain reaction (PCR) and the cycleave real-time quantitative PCR technique (SRL Inc, Tokyo, Japan).

The reported upper limit of normal for the diagnosis of NSCLC and upper limit of the percentiles for healthy individuals of serum CYFRA 21–1 as measured by EIA are 3.5 ng/ml and 2.8 ng/ml, respectively [36]. In contrast, the reported upper limit of the percentiles for healthy individuals of serum CYFRA 21–1 measured by the CLEIA method is 1.6 ng/ml [37], a lower value as compared to that set for measurement by the EIA method. Therefore, for our study, we set the cutoff value for CYFRA 21–1 at 2.2 ng/ml, based on the mean value for healthy subjects + 3SD [37], a lower value as compared to that set for measurement by the EIA method. The cutoff value for serum CEA was set at 5.0 ng/ml, which is the upper limit of normal.

A standard evaluation of the patients, including assessment of the medical history, physical examination and routine laboratory tests, was performed before each treatment. All patients were staged based on the International Association for the Study of Lung Cancer (IASLC) TNM (tumor-node-metastasis) classification, 7th edition [38].

Statistical methods

There were no missing data in our study. Survival was estimated using the Kaplan-Meier method. Overall survival was measured from the date of the first course of the initial therapy to the date of death or that of the last follow-up examination. A log-rank test was performed to evaluate the significance of differences in the overall survival among the groups. P values < 0.05 were considered to be indicative of statistical significance. A multivariate analysis using the Cox proportional hazards model was used to establish the association between the clinical variables and survival. All statistical analyses were carried out using SPSS, version 11.0 for Windows (SPSS Inc., Chicago, IL, USA). To reduce the potential bias arising from some patients dying too early to receive initial therapy, the two patients who died within a month (30 days) of the start of initial therapy were excluded from the analysis.

Results

The cohort consisted of 284 patients who were diagnosed as having stage IIIB or IV lung adenocarcinoma and had received initial therapy.

The clinical characteristics of the patients are summarized in Table 1. The median patient age prior to the start of initial therapy was 65 years (range, 23 to 87 years). The patients were predominantly younger than 70 years of age (81%), the ECOG PS was 0–2 in 93% of patients, and 91% of the patients had stage IV disease. While the lung adenocarcinoma patients with EGFR mutations were predominantly female (64%) and non-smokers (71%), those with wild-type EGFR were predominantly male (77%) and smokers (76%).

Table 1

Patient characteristics

Characteristic	Mt + (n= 121)		Mt – (n= 163)		All (n= 284)
	No.	%	No.	%	No.	%
Age, years
Median (range)	66 (32–87)		65 (23–83)		65 (23–87)
< 70	97	80	134	82	231	81
≥ 70
	24	20	29	18	53	19
Gender
Male	43	36	125	77	168	59
Female	78	64	38	23	116	41
ECOG PS
0-1	103	85	135	83	238	84
> 2	18	15	28	17	46	16
Smoking status
Yes	50	41	124	76	174	61
No	71	59	39	24	110	39
Stage
IIIB	6	5	19	12	25	9
IV	115	95	144	88	259	91
EGFR mutation
Exon 19 deletion	59	49			59	21
Exon 21 L858R	57	47			57	20
Exon 18 G719X	5	4			5	2
Wild type			163	100	163	57
PCV
Median (range)	1.6 (0.1-110.0)		2.3 (0.1-80.0)		2.0 (0.1-110.0)
< 2.2 ng/ml	72	60	78	48	150	53
≥ 2.2 ng/ml	49	40	85	52	134	47
CEA
Median (range)	8 (0.7-11942)		7 (0.5-14985)		7.4 (0.5-14985)
< 5.0 ng/ml	45	37	63	39	108	38
≥ 5.0 ng/ml	76	63	100	61	176	62

EGFR: epidermal growth factor receptor, Mt+: mutant EGFR, Mt-: wild-type EGFR, PCV: pretreatment CYFRA 21–1 value.

Details about the first-line chemotherapy were available for 284 patients including both patient groups with wild-type (Mt-) and mutant EGFR (Mt+) groups (Table 2). About 40% of the EGFR mutation-positive patients received EGFR-TKIs as the initial treatment.

Table 2

Summary of initial treatment delivered among 284 patients

EGFR mutation	Mt – (n= 163)				Mt + (n= 121)
	IIIB		IV		IIIB		IV
	(n= 19)		(n= 144)		(n= 6)		(n= 115)
	No.	%	No.	%	No.	%	No.	%
Treatment
Platinum doublet	4	3	114	70	2	2	54	45
Monotherapy	0		30	18	0		11	9
EGFR-TKI	0		0		0		50	41
Chemoradiotherapy	15	9	0		4	3	0
Specific regimens
Cisplatin-pemetrexed	1		24	15	1		9	7
Carboplatin-paclitaxel	3		52	32	0		27	22
Carboplatin-paclitaxel+ bev	0		2		0		2
Other platinum doublets	0		36	22	1		12	10
Gefitinib	0		0		0		41	34
Erlotinib	0		0		0		7	6
Docetaxel	0		16	10	0		3
Vinorelbine	0		5		0		2
Others	0		24	15	0		6

Mt+: mutant EGFR, Mt-: wild-type EGFR, bev: bevacizumab.

Carboplatin-paclitaxel, the treatment of choice across both groups, was administered to half of the platinum doublet cohort in the Mt- patient group. Meanwhile, docetaxel was administered to half of the monotherapy cohort in the same patient group. However, cisplatin-pemetrexed was the most common regimen of second choice across both the Mt+ and Mt- groups.

The EGFR-TKI used for each treatment line in the Mt+ group is shown in Table 3. Forty-one (58%) patients received gefitinib, while 16 (22%) received erlotinib as first- or second-line treatment in the Mt+ group with PCV (<2.2 ng/ml). Thirty-seven (73%) patients received gefitinib, and 10 (20%) patients received erlotinib as first- or second-line treatment in the Mt+ group with PCV (≥2.2 ng/ml). Of the 121 patients in the Mt+ group, 27 did not receive gefitinib at any treatment-line stage of treatment; among these 27 patients, 19 received erlotinib (6 as first-line, 10 as second-line, 1 as third-line and 2 as further-line treatment). In the Mt+ group, a total of 113 patients (93%) received EGFR-TKIs, while 8 patients did not receive EGFR-TKIs at any stage of treatment. Furthermore, of the 160 patients in the Mt- group, 30 patients received EGFR-TKIs (11 as second-line, 7 as third-line, 6 as fourth-line, 3 as fifth-line, 1 as sixth-line, 1 as seventh-line, and 1 as eighth-line treatment). Fifty-three patients (18%) were still alive at the time of the analysis. The median follow-up period for determining the survival was 39.3 (range; 11.8-84.9) months after the start of initial therapy. The clinical variables identified by univariate analysis to be associated with significantly better survival (Table 4) included female gender (MST 32.4 months versus 20.1 months in males: p = .0086), no smoking history (33.4 months versus 20.1 months in smokers, p = .0012), ECOG PS (0–1) (29.5 months versus 7.9 months in those with a PS of 2–3, p < .0001), presence of EGFR mutation (39.2 months versus 17.8 months in patients without EGFR mutations, p < .0001), PCV < 2.2 ng/ml (38.6 months versus 15.0 months in those with PCV ≥ 2.2 ng/ml, p < .0001), serum CEA < 5.0 ng/ml (32.6 months versus 21.0 months in those with serum CEA ≥ 5.0 ng/ml, p = .036), start date of initial therapy before April 1, 2008 (34.1 months versus 19.3 months in the group that received the initial therapy after April 1, 2008, p = .003) and EGFR-TKI treatment (33.7 months versus 15.3 months in the group not treated with EGFR-TKIs, p < .0001). Multivariate analysis identified EGFR mutation positivity (HR 0.53; 95% CI: 0.34-0.84, p = .0069) and PCV < 2.2 ng/ml (HR 0.43; 95% CI: 0.31-0.59, p < .0001) as independent favorable prognostic factors. Another factor that was found to be an independent prognostic indicator of overall survival was the PS (Table 4). The overall survival rates of patients with advanced lung adenocarcinoma with/ without EGFR mutation are shown in Figure 2. Among the Mt+ patients, the prognosis was more favorable in the group with PCV < 2.2 ng/ml (n = 70) than in the group with PCV > 2.2 ng/ml (n = 48) (median survival time [MST]: 67.0 vs. 21.0 months, p < 0.0001). Among the patients with Mt- also, the prognosis was more favorable in the group with PCV < 2.2 ng/ml (n = 78) than in the group with PCV ≥ 2.2 ng/ml (n = 86) (MST: 24.1 vs. 10.2 months, p < 0.0001).

Table 3

Summary of EGFR-TKI delivered among EGFR mutation positive patients

	EGFR mutation positive
	Low PCV				High PCV
	(< 2.2 ng/ml) (n= 72)				(≥ 2.2 ng/ml) (n= 49)
	Gefitinib		Erlotinib		Gefitinib		Erlotinib
	No.	%	No.	%	No.	%	No.	%
First-line	20	28	5	7	23	47	2	4
Second-line	21	29	11	15	14	29	8	16
Third-line	9	12	6	8	3	6	4	8
Further-line	2	3	14	20	2	4	4	8
Unadministered	20	28	36	50	7	14	31	63

PCV: pretreatment CYFRA 21–1 value.

Table 4

Variables associated with overall survival among 284 patients

Co-variable	No.	Univariate analysis		Multivariate analysis
		MST (months)	P	Variate	OR	95% CI	P
Age
< 70	231	22.8
> 70	53	24.3	0.625
Gender
Male	168	20.1
Female	116	32.4	0.0086	Female	1.06	0.75-1.58	0.75
Smoking status
Yes	174	20.1
No	110	33.4	0.0012	No smoking status	0.84	0.52-1.24	0.39
ECOG PS
0-1	238	29.5
>2	46	7.9	<.0001	PS 0-1	0.34	0.24-0.50	<.0001
Stage
IIIB	25	30.2
IV	259	22.5	0.269
EGFR mutation
Mt (+)	121	39.2
Mt (−)	163	17.8	<.0001	Mutant EGFR	0.53	0.34-0.84	0.0069
PCV
< 2.2 ng/ml	150	38.6
≥ 2.2 ng/ml	134	15.0	<.0001	< 2.2 ng/ml	0.43	0.31-0.59	<.0001
CEA
< 5.0 ng/ml	108	32.6
≥ 5.0 ng/ml	176	21.0	0.036	< 5.0 ng/ml	0.93	0.67-1.26	0.63
Start dates of IT
Before 1/ 4/ 2008	79	34.1		After 1/ 4/ 2008
After 1/ 4/ 2008	205	19.3	0.0030		0.73	0.50-1.15	0.07
EGFR-TKI treatment
Yes	143	33.7
No	141	15.3	<.0001	Yes	0.76	0.50-1.15	0.20

IT: initial therapy, PCV: pretreatment CYFRA 21–1 value, Mt(+): mutant EGFR, M(−): wild-type EGFR.

Figure 2

Kaplan-Meier curves for overall survival in four groups, EGFR mutation status- stratified by PCV. M+: mutant EGFR, M-: wild-type EGFR, PCV: pretreatment CYFRA 21–1 value.

Discussion

In the present study, we demonstrated PCV and EGFR mutation status as independent prognostic factors in untreated advanced lung adenocarcinoma patients. We also showed that PCV < 2.2 ng/ml was a predictor of a favorable outcome in both advanced lung adenocarcinoma patients with wild-type and mutant EGFR.

Serum CYFRA 21–1 has been reported as a prognostic factor in patients with a variety of cancer types, including resectable NSCLC [39,40], biliary tract cancer [41], urothelial cancer [42], head and neck cancer [43], esophageal cancer [44], and cervical cancer [45].

A meta-analysis of CYFRA 21–1 as a prognostic indicator in advanced NSCLC patients showed that the PCV may be a reliable prognostic factor [29], however, since non-adenocarcinoma accounted for 65% of the cases and squamous cell carcinoma for 50%, the role of serum CYFRA 21–1 as a prognostic indicator in the lung adenocarcinoma population remained unclear. Moreover, in a study of PCV as a prognostic indicator in advanced NSCLC patients in whom gefitinib was used as 3rd-line or later therapy, adenocarcinoma accounted for fewer than a half of the cases (47%) [30]. The EGFR mutation status was not included as a variable in the analysis, and the test population was small, consisting of only 50 patients.

Several factors may have contributed to identification of serum CYFRA 21–1 as a prognostic indicator in the advanced lung adenocarcinoma population in the present study. First, there could be a relationship between the serum levels of CYFRA 21–1 and the microfilament formation trend in the tumor cells [22]. CKs are the principal structural elements of intracellular microfilaments. Microfilaments have been shown to be heteropolymers formed from type I and type II keratins which form the cytoskeleton. Moreover, while the CKs (CKs 1, 2, 10/11), on which the degree of keratinization within tumors depends, are strongly expressed in well-differentiated squamous cell carcinomas, they are not detected in the serum. The possibility that they are preferentially removed by macrophages because of their poor solubility has been suggested as the reason for the failure to detect them in the serum [46]. By contrast, soluble CK19 is degraded by tumor lysis and tumor necrosis and released into the blood. Therefore, serum levels of CK19 may indicate the degree of cytoskeleton formation by microfilaments within the tumor cells. Second, there may also be a relationship between serum CYFRA 21–1 levels and the degree of tumor differentiation towards squamous epithelium. CKs with a relatively high molecular mass tend to be associated with differentiation into squamous cell carcinoma, while CKs with a relatively low molecular mass tend to be associated with differentiation into adenocarcinoma [47]. In a study in which monoclonal antibodies were used, the number of cells containing CK19 increased with decreasing degree of differentiation into squamous cell carcinoma, and the presence of intracellular CK19 was consistently demonstrated in pure lung adenocarcinomas [25]. On the other hand, a negative correlation between intracellular CK19 expression and serum CYFRA 21–1 levels has also been shown [24]. Increase in the serum level of CYFRA 21–1 may also be the result of a greater degree of degradation and release of intracellular CK19 into the serum with an increasing tendency towards differentiation into squamous cell carcinoma.

Because identical EGFR mutations have been seen in both the adenocarcinoma component and squamous cell carcinoma component in resected cases of adenosquamous carcinoma [48], it has been suggested that the two components may arise from a single clone [48,49]. Resected cases of adenosquamous carcinoma have been reported to account for 3% of all cases of NSCLC [50], and adenosquamous carcinoma patients have also been reported to have a poor prognosis [51]. The prognosis of patients in whom the tumor tissue consists of a mixture of mutant EGFR cells and wild-type EGFR cells has been reported to be inferior to that of patients with tumors consisting of only mutant EGFR cells, and intratumor heterogeneity has also been investigated [52]. On the other hand, there is a report suggesting that no intratumor heterogeneity of EGFR expression is found in mutant EGFR lung adenocarcinomas, and also that no disparity is found between the EGFR mutation status of the primary tumor and lymph node metastasis [53].

There are several limitations of the present study. The first is that it was a retrospective study conducted at a single institution, and the possibility of a selection bias is undeniable. The prognosis of patients who received initial therapy before April 1, 2008 was significantly superior to that of those who received their initial therapy after 2008. Because we started to perform EGFR mutation analysis in routine clinical practice from April 1, 2008, there is the possibility of a selection bias towards patients who received the initial therapy before April 1, 2008. This is one of the major limitations of our retrospective study. Some studies have reported that EGFR mutations may be a positive prognostic factor for survival in advanced NSCLC patients, regardless of EGFR-TKI therapy [54,55]. Also in the BR.21 trial, the median survival time was reported to be longer in patients with mutant EGFR as compared to that in patients with wild-type EGFR [56]. Although mutant EGFR patients not treated with EGFR-TKIs were found to be a confounding factor, we performed adjustment for the confounding factor using a Cox proportional hazards model. According to the univariate analysis, the date of start of the initial therapy (before April 1, 2008) was a favorable prognostic factor. However, PCV < 2.2 ng/ml, EGFR mutation positivity and PS 0–1 were found to be independent favorable prognostic factors after adjustment for the date of start of the initial therapy. In this study, while the MST (39.2 months) in the mutant EGFR group was not favorable as compared to previous reports [57], the mutant EGFR group with PCV < 2.2 ng/ml had a more favorable prognosis than that of the mutant EGFR group with PCV ≥ 2.2 ng/ml. The proportion of patients who received erlotinib was less in the group with PCV ≥ 2.2 ng/ml than in the group with PCV < 2.2 ng/ml, which could have influenced the more favorable prognosis in the group with PCV < 2.2 ng/ml than in the group with PCV ≥ 2.2 ng/ml. All of the patients with advanced lung adenocarcinoma in whom the diagnosis was made after April 1, 2008 were tested for EGFR mutations at the time of the diagnosis, whereas in the patients with other histological types of lung cancer, the testing was performed at the discretion of the attending physician. Second, the follow-up period was inadequate, especially in the mutant EGFR group with PCV < 2.2 ng/ml, and the censored cases were conspicuous. There was also a problem with the stage distribution (there were relatively few stage IIIB cases). Distant metastasis occurred in all of the stage IIIB cases in which local treatment had been performed, and all of the patients with disease recurrence were tested for EGFR mutations. Moreover, significant survival differences in stage IIIB/ IV were not found in the univariate analysis. Furthermore, the treatment regimens used in the stage IV cases were not standardized, with each of the attending physicians administering any of the various standard treatments used in routine clinical practice recommended by the guidelines of the Japan Lung Cancer Society.

In advanced lung adenocarcinoma, which may be considered as a generalized systemic disease, it may be particularly difficult to determine the characteristics of an entire heterogeneous tumor by tissue diagnosis alone based on examining just one part of the tumor. Based on the results of the present study, we propose that mutant EGFR patients with serum PCV < 2.2 ng/ml have a better prognosis than the mutant EGFR patients with higher PCV.

Conclusions

The potential applications of PCV measurements might include identification of candidates in whom it might have some prognostic value. Furthermore, PCV might be regarded as a routine demographic variable having prognostic value in patients with advanced lung adenocarcinoma.

Abbreviations

NSCLC: Non-small cell lung cancer; PCV: Pretreatment serum CYFRA 21–1 levels; pts: patients; EGFR: Epidermal growth factor receptor; Mt+: Mutant EGFR; Mt-: Wild-type; TKI: Tyrosine kinase inhibitor; CK: Cytokeratin; ECOG PS: Eastern Cooperative Oncology Group performance status; CLEIA: Chemiluminescence enzyme immunoassay; PCR: Polymerase chain reaction; IASLC: International Association of the Study of Lung Cancer; TNM: Tumor-node-metastasis.

Competing interests

The authors have no competing interests to declare.

Authors’ contributions

AO contributed to the drafting of this manuscript and data collection, and KM contributed to the study design and statistical analysis. TT, HA, TS, TT, HK, TN, HM, TN, ME, NY contributed to analysis of the data and interpretation of the findings. All authors have read and approved of the submission of the final manuscript.

Pre-publication history

The pre-publication history for this paper can be accessed here:

http://www.biomedcentral.com/1471-2407/13/354/prepub