集胞藻的随机插入诱变和光激活异养突变株的筛选

以4－碱基限制性内切酶部分酶切集胞藻PCC6803基因文库总质粒DNA,并插入卡那霉素抗性基因标记,构建了二级随机插入诱变文库。以该诱变文库总DNA转化集胞藻PCC6803,得到大量有抗性标记基因随机插入的转化子,利用这一方法获得了不能进行光激活异养生长的突变株,并克隆了抗性标记基因插入部位DNA片段,在持续光照但加DCMU抑制光合作用的情况下,这些突变株仍然能够利用葡萄糖异养生长,推测突变基因与短时光信号的感应有关。     

The structure of genetically modified iron-sulfur cluster Fx in photosystem I as determined by X-ray absorption spectroscopy

Photosystem I (PS I) mediates light-induced electron transfer from P700 through a chlorophyll a, a quinone and a [4Fe-4S] iron-sulfur cluster F_X, located on the core subunits PsaA/B to iron-sulfur clusters F_A/B on subunit PsaC. Structure function relations in the native and in the mutant (psaB-C565S/D566E) of the cysteine ligand of F_X cluster were studied by X-ray absorption spectroscopy (EXAFS) and transient spectroscopy. The structure of F_X was determined in PS I lacking clusters F_A/B by interruption of the psaC2 gene of PS I in the cyanobacterium Synechocystis sp PCC 6803. PsaC-deficient mutant cells assembled the core subunits of PS I which mediated electron transfer mostly to the phylloquinone. EXAFS analysis of the iron resolved a [4Fe-4S] cluster in the native PsaC-deficient PS I. Each iron had 4 sulfur and 3 iron atoms in the first and second shells with average Fe-S and Fe-Fe distances of 2.27 Å and 2.69 Å, respectively. In the C565S/D566E serine mutant, one of the irons of the cluster was ligated to three oxygen atoms with Fe-O distance of 1.81 Å. The possibility that the structural changes induced an increase in the reorganization energy that consequently decreased the rate of electron transfer from the phylloquinone to F_X is discussed.     

集胞藻PCC6803光激活异养生长必需基因s110886的研究

集胞藻PCC6803能够在微弱、短时光刺激的条件下利用葡萄糖进行异养生长,称为光激活异养生长(LAHG)。从其随机插入诱变文库中,筛选到3个不能进行光激活异养生长的突变株,通过反向PCR和测序确定突变基因全部为s110886。将s110886克隆到表达载体pET21-b,在大肠杆菌BL21(DE3)诱导表达,并对产物进行了纯化。用Western印迹法研究s110886在集胞藻PCC6803的表达情况,发现在完全黑暗和光照情况下,其表达水平几乎没有差异,并证明其编码产物分布于膜上。因此,s110886是一个编码膜蛋白的不受光调控的LAHG基因。     

Oxidative stress and metal ions effects on the cores of phycobilisomes in Synechocystis sp. PCC 6803

Inactivation of the chlN gene in Synechocystis sp. PCC 6803 resulted in no chlorophyll and photosystems when the mutant was grown in darkness, providing an in vivo system to study the structure and function of phycobilisomes (PBSs). The effects of hydrogen peroxide (H2O2) and metal ions on the mutant PBSs in vivo were investigated by low temperature fluorescence emission measurement. H2O2 induced an obvious disassembly of the cores of PBSs and interruption of energy transfer from allophycocyanin to the terminal emitter. Among many metal ions only silver induced disassembly of the cores of PBSs. Our results demonstrated for the first time that the cores of PBSs act as targets in vivo for oxidative stress or silver induced damage.