Schaffner C; Laasch H; Hagemann R 1995
- Authors: Schaffner C; Laasch H; Hagemann R
- Title: Detection of point mutations in chloroplast genes of
Antirrhinum majus L. I. Identification of a point
mutation in the psaB gene of a photosystem I plastome mutant.
- Location: Molecular & General Genetics 1995 Dec 15;249(5):533-44
- Abstract: A point mutation in the plastome-encoded psaB gene of the mutant
en:alba-1 of Antirrhinum majus L. was identified by an
analysis of chloroplast DNA with a modified PCR-SSCP technique.
Application of this technique is indicated when a gene or a group of
genes is known in which the point mutation is located. Analysis of
primary photosynthetic reactions in the yellowish white plastome mutant
indicated a dysfunction of photosystem (PS) I. The peak wavelength of PS
I-dependent chlorophyll (Chl) fluorescence emission at 77 K was shifted
by 4 nm to 730 nm, as compared to fluorescence from wild-type. There were
no redox transients of the reaction center Chl P700 upon illumination of
leaves with continuous far-red light or with rate-saturating flashes of
white light. The PS I reaction center proteins PsaA and PsaB are not
detectable by SDS-PAGE in mutant plastids. Hence, plastome encoded PS I
genes were regarded as putative sites of mutation. In order to identify
plastome mutations we developed a modified SSCP (single-strand
conformation polymorphism) procedure using a large PCR fragment which can
be cleaved with various restriction enzymes. When DNA from wild-type and
en:alba-1 was submitted to SSCP analysis, a single stranded HinfI
fragment of a PCR product of the psaB gene showed differences in
electrophoretic mobility. Sequence analysis revealed that the observed
SSCP was caused by a single base substitution at codon 136 (TAT-->TAG) of
the psaB gene. The point mutation produces a new stop codon that leads to
a truncated PsaB protein. The results presented indicate that the
mutation prevents the assembly of a functional PS I complex. The
applicability to other plastome mutants of the new method for detection
of point mutations is discussed.
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