Rak J W, McEachern D, Miller F R
Breast Cancer Biology Program, Michigan Cancer Foundation, Detroit 48201.
Br J Cancer. 1992 May;65(5):641-8. doi: 10.1038/bjc.1992.138.
A sequential, quantitative loss of Peanut agglutinin (PNA) binding with progression of mouse mammary cells from normal to preneoplastic to neoplastic phenotypes was observed. Normal mammary epithelium, preneoplastic mammary lesions designated D2HAN (D2-type hyperplastic alveolar nodules) and a series of nine spontaneous tumours (D2ST1, D2ST2, D2ST3, D2ST4, D2A1, D2F2, D2.0R, D2.1, EMT6R08) derived from mice bearing D2HAN were grown in culture and analysed by flow cytometry with respect to PNA binding intensity to the cell surface. Primary cultures of normal mammary epithelium strongly bound PNA. A stepwise decrease in PNA binding by preneoplastic D2HAN cells and subsequent tumours arising from those hyperplastic lesions was observed. Three cloned tumour subpopulations derived from such tumours exhibited dramatic differences in PNA binding ranging from high (D2.0R) to low (D2.1) to very low (D2A1 cells). Their growth rate in vitro was similar. However, an inverse correlation between PNA binding and malignant characteristics, such as the incidence and latency of subcutaneous tumours and the efficiency of the tumour cells to form lung colonies after i.v. injection, existed. Cells subsequently derived from tumours resulting from injection of the D2.0R clone (high PNA binding, low tumorigenicity) were found to have diminished PNA binding properties and to be more tumorigenic when reimplanted into syngeneic mice. The difference in PNA binding (up to 50-fold) between normal mammary cells and other mouse mammary tumour cells, i.e., unrelated to D2HAN lesions, was also seen. These include six sister subpopulations derived from a single BALB/cfC3H mouse mammary tumour (lines: 67, 66c14, 168FARN, 4TO7, 68H, 64pT) as well as SP1 spontaneous CBA/J mouse mammary carcinoma. The difference was greatly reduced by neuraminidase treatment suggesting a masking of PNA binding sites by sialic acid. Separation of cell lysates by SDS-PAGE revealed a high molecular weight PNA binding glycoprotein (greater than 250 kd) expressed by normal mammary epithelium and preneoplastic D2HAN cells, but not by tumour cells regardless of neuraminidase treatment. A PNA reactive glycoprotein of approximately 90 kd was uniquely expressed in normal mammary epithelial lysates, although neuraminidase treatment exposed a similar band in a few tumour lines. Normal mammary epithelium, preneoplastic D2HAN cells, and the poorly tumorigenic clone D2.0R expressed a PNA binding glycoprotein of approximately 150 kd. This band appeared to be specifically sialylated during transition from the high PNA binding, low tumorigenic phenotype of D2.0R cells to the low PNA binding, highly tumorigenic phenotype of cells isolated from tumours resulting from s.c. implantation of D2.0R cells.(ABSTRACT TRUNCATED AT 400 WORDS)
观察到随着小鼠乳腺细胞从正常表型发展为癌前表型再到肿瘤表型,花生凝集素(PNA)结合呈现出顺序性的定量减少。将正常乳腺上皮、指定为D2HAN(D2型增生性肺泡结节)的癌前乳腺病变以及源自携带D2HAN小鼠的一系列九个自发肿瘤(D2ST1、D2ST2、D2ST3、D2ST4、D2A1、D2F2、D2.0R、D2.1、EMT6R08)在培养物中生长,并通过流式细胞术分析其细胞表面PNA结合强度。正常乳腺上皮的原代培养物与PNA强烈结合。观察到癌前D2HAN细胞以及由这些增生性病变产生的后续肿瘤的PNA结合呈逐步下降。源自此类肿瘤的三个克隆肿瘤亚群在PNA结合方面表现出显著差异,范围从高(D2.0R)到低(D2.1)再到非常低(D2A1细胞)。它们在体外的生长速率相似。然而,PNA结合与恶性特征之间存在负相关,如皮下肿瘤的发生率和潜伏期以及静脉注射后肿瘤细胞形成肺集落的效率。随后从注射D2.0R克隆(高PNA结合,低致瘤性)产生的肿瘤中获得的细胞,在重新植入同基因小鼠时,其PNA结合特性降低且致瘤性更强。正常乳腺细胞与其他小鼠乳腺肿瘤细胞(即与D2HAN病变无关)之间也存在PNA结合差异(高达50倍)。这些包括源自单个BALB/cfC3H小鼠乳腺肿瘤的六个姐妹亚群(系:67、66c14、168FARN、4TO7、68H、64pT)以及SP1自发CBA/J小鼠乳腺癌。神经氨酸酶处理大大降低了这种差异,表明唾液酸掩盖了PNA结合位点。通过SDS-PAGE分离细胞裂解物显示,正常乳腺上皮和癌前D2HAN细胞表达一种高分子量PNA结合糖蛋白(大于250 kd),而无论神经氨酸酶处理如何,肿瘤细胞均不表达。正常乳腺上皮裂解物中独特表达一种约90 kd的PNA反应性糖蛋白,尽管神经氨酸酶处理在一些肿瘤系中也暴露了类似条带。正常乳腺上皮、癌前D2HAN细胞以及低致瘤性克隆D2.0R表达一种约150 kd的PNA结合糖蛋白。在从D2.0R细胞的高PNA结合、低致瘤性表型转变为皮下植入D2.0R细胞产生的肿瘤中分离出的细胞的低PNA结合、高致瘤性表型的过程中,这条带似乎发生了特异性唾液酸化。(摘要截断于400字)
