Connors M J, Setlow P
J Bacteriol. 1985 Jan;161(1):333-9. doi: 10.1128/jb.161.1.333-339.1985.
The first Bacillus subtilis small, acid-soluble spore protein (SASP) gene has been cloned by using previously cloned B. megaterium SASP genes as DNA-DNA hybridization probes. Determination of the DNA sequence of the B. subtilis SASP gene showed that it codes for a 72-residue protein (termed SASP-1) containing a single spore protease cleavage site as well as other sequences conserved in Bacillus megaterium SASPs A, C, C-1, C-2, and C-3. The B. subtilis SASP-1 genes's coding sequence is preceded by a potential Bacillus ribosome-binding site, and is followed by a sequence that could form a stem-and-loop structure characteristic of transcription termination sites. Upstream from the coding sequence there are no obvious homologies with other B. subtilis sporulation genes, but similarities with B. megaterium SASP genes are evident. SASP-1 mRNA (290 bases long) is absent from vegetative cells, but appears midway in sporulation and then disappears. The cloned SASP-1 gene hybridizes to three bands other than the SASP-1 gene itself in EcoRI or HindIII digests of B. subtilis DNA. Presumably these other bands represent SASP genes related to the SASP-1 gene, and we have been able to detect at least three such proteins in B. subtilis spores.
利用先前克隆的巨大芽孢杆菌小酸溶性芽孢蛋白(SASP)基因作为DNA-DNA杂交探针,已克隆出首个枯草芽孢杆菌的SASP基因。对枯草芽孢杆菌SASP基因的DNA序列测定表明,它编码一种含72个氨基酸残基的蛋白质(称为SASP-1),该蛋白质含有一个单一的芽孢蛋白酶切割位点以及在巨大芽孢杆菌SASP A、C、C-1、C-2和C-3中保守的其他序列。枯草芽孢杆菌SASP-1基因的编码序列之前有一个潜在的芽孢杆菌核糖体结合位点,之后是一个可形成转录终止位点特征性茎环结构的序列。在编码序列上游,与其他枯草芽孢杆菌芽孢形成基因没有明显的同源性,但与巨大芽孢杆菌SASP基因的相似性很明显。营养细胞中不存在SASP-1 mRNA(长290个碱基),但在芽孢形成过程中中期出现,然后消失。在枯草芽孢杆菌DNA的EcoRI或HindIII酶切片段中,克隆的SASP-1基因除了与SASP-1基因本身杂交外,还与另外三条带杂交。推测这些其他条带代表与SASP-1基因相关的SASP基因,并且我们已经能够在枯草芽孢杆菌芽孢中检测到至少三种这样的蛋白质。
