Clarke A E, Anderson M A, Bacic T, Harris P J, Mau S L
J Cell Sci Suppl. 1985;2:261-85. doi: 10.1242/jcs.1985.supplement_2.14.
The molecular basis of recognition between plant cells is incompletely understood. Some principles established for recognition between animal cells may well apply to plant cell recognition, although, in contrast to animal cells, plant cells are encased by cell walls that play an active role in plant cell-cell recognition. The interaction that controls fertilization in flowering plants involves recognition between pollen or pollen tubes and the female sexual tissues. In many flowering plant families, self-incompatibility (S) genes operate to prevent inbreeding. In plants that have gametophytically controlled self-incompatibility, recognition of common S alleles in pollen tube and style results in arrest of pollen tube growth within the style. Self-incompatibility therefore provides a model cell-cell recognition system that is genetically defined. We have taken two approaches to defining cell recognition involved in gametophytic self-incompatibility in Nicotianas alata. Firstly, we have established the major features of the pollen tube wall and the matrix of the style transmitting tissue that are in contact with the growing pollen tube. Secondly, we have established the nature of style glycoproteins that are associated with the S genotype and have initiated a program to clone the genes coding for the protein component of these glycoproteins. Analyses of the pollen tube are consistent with the major polymers being a (1----3)-beta-D-glucan (callose) and a (1----5)-alpha-L-arabinan. The pollen tube has two distinct layers: gold immunocytochemistry using a monoclonal antibody directed to terminal alpha-L-arabinosyl residues shows the binding is confined to the outer layers. The major component of the extracellular matrix of the style transmitting tissue is a family of proteoglycans, the arabinogalactan-proteins. A major glycoprotein that segregates with the S2 allele is present in extracts of mature styles. This component has a high pI (greater than 9.5) and an apparent molecular weight of 32 X 10(3). It is not present in extracts of immature styles of N. alata genotypes bearing the S2 allele, or in extracts from other organs of N. alata or styles of other members of the Solanaceae. The isolated glycoprotein is an effective inhibitor of in vitro pollen tube growth. This evidence suggests that the S2-associated glycoprotein is either the product of the S2 allele, or a gene closely associated with the S gene. We have prepared a cDNA library from styles of one genotype and are screening this library with mRNA from mature and immature styles.(ABSTRACT TRUNCATED AT 400 WORDS)
植物细胞间识别的分子基础尚未完全明晰。一些已确立的动物细胞间识别原则很可能适用于植物细胞识别,不过,与动物细胞不同,植物细胞被细胞壁包裹,细胞壁在植物细胞间识别中发挥着积极作用。控制开花植物受精的相互作用涉及花粉或花粉管与雌性功能组织之间的识别。在许多开花植物科中,自交不亲和(S)基因发挥作用以防止近亲繁殖。在具有配子体控制的自交不亲和的植物中,花粉管和花柱中共同S等位基因的识别会导致花粉管在花柱内生长停滞。因此,自交不亲和提供了一个由基因定义的细胞间识别系统模型。我们采用了两种方法来确定参与烟草配子体自交不亲和的细胞识别。首先,我们确定了与生长中的花粉管接触的花粉管壁和花柱传递组织基质的主要特征。其次,我们确定了与S基因型相关的花柱糖蛋白的性质,并启动了一个程序来克隆编码这些糖蛋白蛋白质成分的基因。对花粉管的分析表明,主要聚合物是一种(1→3)-β-D-葡聚糖(胼胝质)和一种(1→5)-α-L-阿拉伯聚糖。花粉管有两个不同的层:使用针对末端α-L-阿拉伯糖基残基的单克隆抗体进行的金免疫细胞化学显示,结合仅限于外层。花柱传递组织细胞外基质的主要成分是一类蛋白聚糖,即阿拉伯半乳聚糖蛋白。一种与S2等位基因共分离的主要糖蛋白存在于成熟花柱的提取物中。该成分具有高pI(大于9.5)和32×10³的表观分子量。它不存在于携带S2等位基因的烟草基因型未成熟花柱的提取物中,也不存在于烟草其他器官或茄科其他成员花柱的提取物中。分离出的糖蛋白是体外花粉管生长的有效抑制剂。这一证据表明,与S2相关的糖蛋白要么是S2等位基因的产物,要么是与S基因紧密相关的基因。我们从一种基因型的花柱中制备了一个cDNA文库,并用成熟和未成熟花柱的mRNA对该文库进行筛选。(摘要截短至400字)
