首页> 外文期刊>BMC Cancer >Improved immunohistochemical evaluation of micrometastases in sentinel lymph nodes of cutaneous melanoma with 'MCW Melanoma Cocktail' – A mixture of monoclonal antibodies to MART-1, melan-A, and tyrosinase
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Improved immunohistochemical evaluation of micrometastases in sentinel lymph nodes of cutaneous melanoma with 'MCW Melanoma Cocktail' – A mixture of monoclonal antibodies to MART-1, melan-A, and tyrosinase

机译:“ MCW黑色素瘤鸡尾酒”改善了皮肤黑色素瘤前哨淋巴结微转移的免疫组织化学评估–一种针对MART-1,黑色素A和酪氨酸酶的单克隆抗体的混合物

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Background MART-1, Melan-A, and Tyrosinase have shown encouraging results for evaluation of melanoma micrometastases in sentinel lymph nodes, as compared to conventionally used S-100 protein and HMB-45. To achieve higher sensitivity, some studies recommend evaluation of three sections, each at intervals of 200 μ. This would mean, routine staining of three adjacent sections in each of the three clusters at intervals of 200 μ, requiring nine slides resulting in added expense. If a cocktail of these antibodies could be used, only one section would be required instead of three generating significant cost savings. Methods We prepared a combination of monoclonal antibodies to these three immunomarkers in optimized dilutions (MART-1, clone M2-7C10, dilution 1:500; Melan-A, clone A103, dilution 1:100; and Tyrosinase, clone T311, dilution 1:50) and designated it as 'MCW melanoma cocktail'. Formalin-fixed paraffin-embedded tissue sections of sentinel lymph nodes from patients with cutaneous melanoma, without macro-metastases were evaluated with this cocktail. Results Melanoma micrometastases were easily detectable with the cocktail in 41 out of 188 slices (8/24 cases). The diagnostic accuracy amongst five pathologists did not show statistically significant difference. Out of 188 slices, 78 had adjacent sections immunostained individually with MART-1 and Melan-A during our previous study. Of these 78 slices, 21 were positive for melanoma micrometastases with MART-1 and Melan-A individually. However, the adjacent section of these slices immunostained with the cocktail detected metastases in four additional slices. Thus, MART-1 and Melan-A could not detect melanoma micrometastases individually in 16% (4/25) of slices positive with the cocktail. Benign capsular nevi were immunoreactive for the cocktail in 4.8% (9/188) slices. All 81 slices of negative test controls (sentinel lymph nodes of mammary carcinoma) were interpreted correctly as negative for melanoma micrometastases. Conclusions The melanoma cocktail facilitated easy interpretation of melanoma micrometastases in sentinel lymph nodes with high interobserver agreement. There was improvement in detection rate with the cocktail as compared to MART-1 and Melan-A individually. Furthermore, this approach facilitates cost savings.
机译:与常规使用的S-100蛋白和HMB-45相比,背景MART-1,Melan-A和酪氨酸酶已显示出令人鼓舞的结果,可用于评估前哨淋巴结中的黑色素瘤微转移。为了获得更高的灵敏度,一些研究建议评估三个切片,每个切片的间隔为200μ。这意味着对三个簇中每个簇的三个相邻部分进行常规染色,间隔为200μ,需要9个载玻片,从而增加了费用。如果可以使用这些抗体的混合物,则只需一个部分,而不是三个部分,可以节省大量成本。方法我们以优化的稀释度制备了针对这三种免疫标记的单克隆抗体组合(MART-1,克隆M2-7C10,稀释度1:500; Melan-A,克隆A103,稀释度1:100;酪氨酸酶,克隆T311,稀释度1 :50),并将其命名为“ MCW黑色素瘤鸡尾酒”。用这种鸡尾酒液评估了福尔马林固定的石蜡包埋的无黑色素瘤皮肤黑素瘤患者前哨淋巴结的组织切片。结果在188片切片中,有41份(8/24例)的鸡尾酒容易检测到黑色素瘤微转移。五位病理学家的诊断准确性未显示统计学上的显着差异。在我们先前的研究中,在188个切片中,有78个切片分别用MART-1和Melan-A免疫染色。在这78个切片中,有21个分别带有MART-1和Melan-A的黑色素瘤微转移阳性。然而,用鸡尾酒免疫染色的这些切片的相邻部分在另外四个切片中检测到转移。因此,MART-1和Melan-A无法在鸡尾酒阳性的16%(4/25)切片中单独检测到黑色素瘤微转移。良性荚膜痣对4.8%(9/188)切片的鸡尾酒具有免疫反应性。所有81片阴性测试对照(乳腺前哨淋巴结)正确解释为黑色素瘤微转移阴性。结论黑色素瘤混合物有助于在观察者之间达成较高共识的前哨淋巴结中容易地解释黑色素瘤微转移。与单独的MART-1和Melan-A相比,该鸡尾酒的检测率有所提高。此外,这种方法有助于节省成本。

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