IL-9 Is a Biomarker of BIA-ALCL Detected Rapidly by Lateral Flow Assay.

IF 3 2区 医学 Q1 SURGERY Aesthetic Surgery Journal Pub Date : 2024-11-15 DOI:10.1093/asj/sjae137
Peng Xu, Katerina Kourentzi, Richard Willson, Honghua Hu, Anand Deva, Patricia McGuire, Caroline Glicksman, Marshall Kadin
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Abstract

Background: A delayed seroma around breast implants is the most common clinical presentation of breast implant-associated anaplastic large cell lymphoma (BIA-ALCL). Interleukin-9 (IL-9), IL-10, and IL-13 concentrations are significantly higher in BIA-ALCL than in benign seromas, offering a means to distinguish between these conditions.

Objectives: The aim of this research was to test the ability of a lateral flow assay (LFA) to detect high concentrations of IL-9 rapidly. In addition, the authors compared CD30 and IL-9 LFAs for distinguishing BIA-ALCL from benign seromas.

Methods: Samples of 26 seromas (15 benign, 11 malignant) were tested on in-house-prepared LFA strips for IL-9 and CD30. Nanoparticle-conjugated antibodies specific to IL-9 and CD30 were used for detection. The intensity of both the test line (TL) and a control line (CL) were analyzed and the TL/CL ratio was calculated. IL-9 protein and IL-9 transcription factor PU.1 were stained in BIA-ALCL lines and clinical samples.

Results: The IL-9 LFA could reliably distinguish BIA-ALCL from benign seromas when the IL-9 concentration was >10 ng/ml. The CD30 LFA was positive in all 11 malignant cases. In 1 case with only faint CD30 and IL-10 TLs, the IL-9 LFA was clearly positive. Immunohistochemistry showed that IL-9 and PU.1 were present in tumor cells in BIA-ALCL lines and clinical samples.

Conclusions: Concentrations of IL-9 >10 ng/ml reliably distinguished BIA-ALCL from benign seromas. Moreover, the IL-9 LFA could detect BIA-ALCL when both the CD30 and IL-10 LFAs were not definitive, suggesting a multiplex LFA measuring IL-9, CD30, and IL-10 might be more effective in detecting BIA-ALCL in selected cases.

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IL-9是通过侧流测定法快速检测出BIA-ALC的生物标记物
背景:乳房植入物周围的迟发性血清肿是 BIA-ALCL 最常见的临床表现。然而,大多数血清肿是由良性原因引起的。因此,必须将良性血清肿与 BIA-ALCL 引起的血清肿区分开来。之前的一项研究发现,BIA-ALC 中 IL-9、IL-10 和 IL-13 的平均浓度明显高于良性血清肿:本研究的目的是测试侧流检测法(LFA)快速检测高浓度 IL-9 的能力。因为我们之前报道过 CD30 LFA 能检测出血清瘤中的 BIA-ALC,所以我们比较了 CD30 和 IL-9 LFA 在区分 BIA-ALCL 和良性血清瘤方面的作用:用内部制备的条带对 26 个血清瘤(15 个良性,11 个恶性)的 30 微升样本进行 IL-9 和 CD30 检测。检测时使用纳米颗粒结合的特异性 IL-9 和 CD30 抗体。IL-9 在未稀释的样本中进行分析,CD30 样本在 1:3 稀释度下进行优化。通过在良性血清瘤中添加重组 IL-9 来确定检测的动态范围。图像分析测量检测线(TL)和对照线(CL)的强度,并计算 TL/CL 比值。对 BIA-ALCL 株系和临床样本中的 IL-9 蛋白和 IL-9 转录因子 PU.1 进行染色:结果:当 IL-9 浓度大于 10 ng/ml 时,IL-9 LFA 能可靠地区分 BIA-ALCL 和良性血清瘤。CD30 LFA 在所有 11 例恶性病例中均呈阳性。在一个只有微弱 CD30 和 IL-10 检测线的病例中,IL-9 LFA 明显呈阳性。免疫组化显示,IL-9及其重要转录因子PU.1存在于BIA-ALCL系和临床样本的肿瘤细胞中:结论:IL-9是BIA-ALCL的一种肿瘤细胞生物标记物,可通过侧流试验和免疫组化法检测到。IL-9浓度大于10纳克/毫升可将BIA-ALC与良性血清肿瘤可靠地区分开。此外,IL-9 LFA能检测出BIA-ALCL,而CD30 LFA不能确定,且IL-10浓度低,IL-10 TL微弱,这表明包括IL-9、CD30和IL-10在内的多重LFA可能更有效地检测特定病例中的BIA-ALCL。
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来源期刊
CiteScore
6.20
自引率
20.70%
发文量
309
审稿时长
6-12 weeks
期刊介绍: Aesthetic Surgery Journal is a peer-reviewed international journal focusing on scientific developments and clinical techniques in aesthetic surgery. The official publication of The Aesthetic Society, ASJ is also the official English-language journal of many major international societies of plastic, aesthetic and reconstructive surgery representing South America, Central America, Europe, Asia, and the Middle East. It is also the official journal of the British Association of Aesthetic Plastic Surgeons, the Canadian Society for Aesthetic Plastic Surgery and The Rhinoplasty Society.
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