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通过荧光杂交检测肺腺癌中的间变性淋巴瘤激酶基因重排时,Diff-Quik染色的细胞学涂片无需脱色。

Destaining of Diff-Quik stained cytologic smears is not necessary for the detection of anaplastic lymphoma kinase gene rearrangement in lung adenocarcinoma by fluorescence hybridization.

作者信息

Xu Weisheng, Khurana Kamal K, Tull Jamie, Maciak Charlene, Zhang Shengle

机构信息

Department of Pathology, State University of New York (SUNY) Upstate Medical University, Syracuse, New York, USA.

出版信息

J Cytol. 2016 Jul-Sep;33(3):154-158. doi: 10.4103/0970-9371.188061.

Abstract

BACKGROUND

Anaplastic lymphoma kinase () gene rearrangement analysis by fluorescence hybridization (FISH) is one of the standard molecular tests for targeted therapy of lung adenocarcinoma. However, insufficient cell block cellularity may impede molecular testing. A recent study showed that Diff-Quik (DQ) stained cytology smear is suitable for by FISH.

AIMS

The aim of our study was to observe the impact of destaining intervals on the quality of FISH signals and determine if DQ smears without destaining would allow FISH analysis.

MATERIALS AND METHODS

Thirty-five DQ smears from 27 cases of lung adenocarcinoma were analyzed for gene rearrangement by FISH. Twenty three DQ smears were destained for different intervals, including 30 s (13 cases), 1 min (6 cases), or 2 min (4 cases). Twelve DQ smears were not subjected to destaining. For further validation, FISH signals in 8 smears and 6 cell blocks were compared with the paired destained DQ smears. The signal quality was semi-quantified and analyzed with Chi-squared test.

RESULTS

Of the total 27 selected cases, three (11%) were positive for gene rearrangement, whereas 24 (89%) were negative. FISH signal was satisfactory in all DQ smears. There was no significant difference in the quality of signal among smears with different destaining intervals ( = 0.55) or between smears with and without destaining ( = 0.41). DQ smears without destaining showed identical FISH results and similar or better signals as compared with paired destained smears and cell blocks in all cases.

CONCLUSIONS

Duration of destaining intervals does not impact the quality of FISH signal on DQ smears. Destaining of DQ smears is not necessary for by FISH.

摘要

背景

通过荧光原位杂交(FISH)进行间变性淋巴瘤激酶(ALK)基因重排分析是肺腺癌靶向治疗的标准分子检测方法之一。然而,细胞块细胞数量不足可能会妨碍分子检测。最近一项研究表明,Diff - Quik(DQ)染色的细胞学涂片适用于FISH检测ALK。

目的

本研究的目的是观察脱色时间间隔对FISH信号质量的影响,并确定未脱色的DQ涂片是否能进行FISH分析。

材料与方法

对27例肺腺癌患者的35张DQ涂片进行FISH分析以检测ALK基因重排。23张DQ涂片进行了不同时间间隔的脱色,包括30秒(13例)、1分钟(6例)或2分钟(4例)。12张DQ涂片未进行脱色。为进一步验证,将8张涂片和6个细胞块中的FISH信号与配对的脱色DQ涂片进行比较。信号质量进行半定量分析,并采用卡方检验。

结果

在总共27例入选病例中,3例(11%)ALK基因重排阳性,而24例(89%)为阴性。所有DQ涂片中FISH信号均令人满意。不同脱色时间间隔的涂片之间信号质量无显著差异(P = 0.55),脱色与未脱色涂片之间也无显著差异(P = 0.41)。在所有病例中,未脱色的DQ涂片显示出与配对的脱色涂片和细胞块相同的FISH结果,且信号相似或更好。

结论

脱色时间间隔的长短不影响DQ涂片上FISH信号的质量。FISH检测ALK时,DQ涂片无需脱色。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/a8d9/4995874/a55a483e2b34/JCytol-33-154-g003.jpg

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