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流式细胞术定量分析晚期头颈癌中增殖相关核抗原p105及DNA含量:RTOG 91-08研究结果

Flow cytometric quantification of the proliferation-associated nuclear antigen p105 and DNA content in advanced head & neck cancers: results of RTOG 91-08.

作者信息

Fu K K, Hammond E, Pajak T F, Clery M, Doggett R L, Byhardt R W, McDonald S, Cooper J S

机构信息

Department of Radiation Oncology, University of California, San Francisco.

出版信息

Int J Radiat Oncol Biol Phys. 1994 Jul 1;29(4):661-71. doi: 10.1016/0360-3016(94)90552-5.

Abstract

PURPOSE

p105 is a proliferation-associated nuclear antigen which identifies proliferating but not resting cells. The objectives of this Radiation Therapy Oncology Group (RTOG) protocol (91-08) were: (1) to correlate tumor proliferative potential estimated using the p105 assay and deoxyribonucleic acid (DNA) analysis with treatment outcome in patients irradiated for advanced squamous cell carcinoma of the head and neck; and (2) to evaluate the potential of p105 labeling indices as a predictive assay.

METHODS AND MATERIALS

Paraffin blocks of pretreatment biopsies of the primary tumor or metastatic neck nodes of patients with Stage III or IV squamous cell carcinoma of the head and neck treated with radiotherapy alone in three previous RTOG protocols (79-13, 79-15, and 83-13) were retrospectively obtained. From these paraffin blocks, areas of tumor were selected based on histological examinations and sectioned. Nuclei suspensions were then prepared and processed for p105 antibody and DNA staining and subsequent flow cytometric quantification of p105 labeling indices and DNA content and correlation with local-regional control and survival.

RESULTS

Paraffin blocks of tumor biopsies from 148 out of a total of 598 eligible patients were available. Of these, 143 were analyzable. The median and (range) of p105 labeling index (LI-C), p105 labeling index of cells in S phase (LI-S), and p105 antigen density (AD) were: 66.6 (3.85-99.5), 9 (1.55-36), and 93.2 (7.4-628.5), respectively. Deoxyribonucleic acid was diploid in 67 (47%), aneuploid in 22 (15%) and mixed aneuploid/diploid in 54 (38%) patients. There was a strong correlation between AD and DNA ploidy. Antigen density was above median in 91.5% of the aneuploid or mixed aneuploid/diploid tumors, but only in 8.5% of the diploid tumors. Patients with aneuploid or mixed aneuploid/diploid tumors had significantly greater local-regional failures than patients with diploid tumors (p = .0180). Those with p105 LI-C below the median or p105 AD above the median also had significantly greater local-regional failures (p = .0500 and p = .0167, respectively). Patients with p105 AD below the median had significantly better survival than those above the median (p = .0444), although there was no significant difference in survival with respect to DNA ploidy or p105 LI-C. Multivariate analyses showed that T-stage (p = .0001) and p105 AD (p = .0044) were significant prognostic factors for local-regional control, and T-stage (p = .0080), N-stage (p = .0021), primary site (p = .0110), and p105 AD (p = .0326) were significant prognostic factors for survival.

CONCLUSION

These results suggest that flow cytometric quantitation of the proliferation-associated nuclear antigen p105 and DNA content of pretreatment tumor biopsies may be a potentially useful predictive assay in patients irradiated for advanced squamous cell carcinomas of the head and neck.

摘要

目的

p105是一种与增殖相关的核抗原,可识别增殖细胞而非静止细胞。放射治疗肿瘤学组(RTOG)方案(91 - 08)的目标是:(1)将使用p105检测和脱氧核糖核酸(DNA)分析评估的肿瘤增殖潜能与接受头颈部晚期鳞状细胞癌放疗患者的治疗结果相关联;(2)评估p105标记指数作为预测检测方法的潜力。

方法和材料

回顾性获取了前三个RTOG方案(79 - 13、79 - 15和83 - 13)中仅接受放射治疗的III期或IV期头颈部鳞状细胞癌患者的原发肿瘤或颈部转移淋巴结预处理活检的石蜡块。从这些石蜡块中,根据组织学检查选择肿瘤区域并进行切片。然后制备细胞核悬液,进行p105抗体和DNA染色,并随后通过流式细胞术定量p105标记指数和DNA含量,并与局部区域控制和生存率相关联。

结果

在总共598名符合条件的患者中,有148名患者的肿瘤活检石蜡块可用。其中,143名可进行分析。p105标记指数(LI - C)、S期细胞的p105标记指数(LI - S)和p105抗原密度(AD)的中位数及(范围)分别为:66.6(3.85 - 99.5)、9(1.55 - 36)和93.2(7.4 - 628.5)。67名(47%)患者的DNA为二倍体,22名(15%)为非整倍体,54名(38%)为非整倍体/二倍体混合。AD与DNA倍性之间存在强相关性。在91.5%的非整倍体或非整倍体/二倍体混合肿瘤中,抗原密度高于中位数,但在二倍体肿瘤中仅为8.5%。非整倍体或非整倍体/二倍体混合肿瘤患者的局部区域失败率明显高于二倍体肿瘤患者(p = 0.0180)。p105 LI - C低于中位数或p105 AD高于中位数的患者局部区域失败率也明显更高(分别为p = 0.0500和p = 0.0167)。p105 AD低于中位数的患者生存率明显高于高于中位数的患者(p = 0.0444),尽管在DNA倍性或p105 LI - C方面生存率无显著差异。多因素分析表明,T分期(p = 0.0001)和p105 AD(p = 0.0044)是局部区域控制的重要预后因素,T分期(p = 0.0080)、N分期(p = 0.0021)、原发部位(p =

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