Poole K, Hancock R E
J Bacteriol. 1986 Mar;165(3):987-93. doi: 10.1128/jb.165.3.987-993.1986.
Bacteria from members of the families Enterobacteriaceae and Pseudomonadaceae were grown under phosphate-deficient (0.1 to 0.2 mM Pi) conditions and examined for the production of novel membrane proteins. Of the 17 strains examined, 12 expressed a phosphate-starvation-induced outer membrane protein which was heat modifiable in that after solubilization in sodium dodecyl sulfate at low temperature the protein ran on gels as a diffuse band of higher apparent molecular weight, presumably an oligomer form, which shifted to an apparent monomer form after solubilization at high temperature. These proteins fell into two classes based on their monomer molecular weights and the detergent conditions required to release the proteins from the peptidoglycan. The first class, expressed by species of the Pseudomonas fluorescens branch of the family Pseudomonadaceae, was similar to the phosphate-starvation-inducible, channel-forming protein P of Pseudomonas aeruginosa. The second class resembled the major enterobacterial porin proteins and the phosphate-regulated PhoE protein of Escherichia coli. Using a protein P-trimer-specific polyclonal antiserum, we were able to demonstrate cross-reactivity of the oligomeric forms of both classes of these proteins on Western blots. However, this antiserum did not react with the monomeric forms of any of these proteins, including protein P monomers. With a protein P-monomer-specific antiserum, no reactivity was seen with any of the phosphate-starvation-inducible membrane proteins (in either oligomeric or monomeric form), with the exception of protein P monomers. These results suggest the presence of conserved antigenic determinants only in the native, functional proteins.
对肠杆菌科和假单胞菌科成员的细菌在缺磷(0.1至0.2 mM无机磷)条件下进行培养,并检测新型膜蛋白的产生。在所检测的17个菌株中,有12个表达了一种磷饥饿诱导的外膜蛋白,该蛋白具有热可修饰性,即在低温下于十二烷基硫酸钠中溶解后,该蛋白在凝胶上呈现为一条较高表观分子量的弥散条带,推测为寡聚体形式,而在高温下溶解后则转变为表观单体形式。根据这些蛋白的单体分子量以及从肽聚糖释放这些蛋白所需的去污剂条件,这些蛋白可分为两类。第一类由假单胞菌科荧光假单胞菌分支的物种表达,类似于铜绿假单胞菌的磷饥饿诱导型通道形成蛋白P。第二类类似于主要的肠杆菌孔蛋白以及大肠杆菌的磷调节PhoE蛋白。使用蛋白P三聚体特异性多克隆抗血清,我们能够在蛋白质印迹上证明这两类蛋白的寡聚体形式具有交叉反应性。然而,该抗血清与这些蛋白的任何单体形式均无反应,包括蛋白P单体。使用蛋白P单体特异性抗血清,除蛋白P单体外,未观察到与任何磷饥饿诱导型膜蛋白(无论是寡聚体还是单体形式)有反应性。这些结果表明仅在天然功能性蛋白中存在保守的抗原决定簇。