Soil fungal community composition at Mars Oasis,a southern maritime Antarctic site,assessed by PCR amplification and cloning

PCR amplification of ITS1-5.8S-ITS2 regions of rDNA followed by cloning was used to determine the fungi present in soil from three sites at Mars Oasis in the southern maritime Antarctic. The soils sampled were adjacent to, or distant from, a meltwater pond, and had moisture contents of 8 %, 3.6 % and 2.5 %. Sequences bearing close similarity to Chytridiales were commonly recorded in clone libraries from the wettest soil. In contrast, sequences from the driest soil matched closely with ectomycorrhizal members of the Helotiales and less closely with Serendipita-like Sebacinales, Tetracladium and ascomycetous black yeasts, such as Rhinocladiella- and Cladophialophora-like fungi and members of the Verrucariales. Sequences loosely similar to Tetracladium, Arrhenia and Omphalina were frequently recovered from the soil of moderate moisture content. Our study corroborates research from the Dry Valleys indicating that soil moisture has an important influence on the composition of Antarctic soil fungal communities.     

PIPKs are essential for rhizoid elongation and caulonemal cell development in the moss Physcomitrella patens

PtdIns‐4,5‐bisphosphate is a lipid messenger of eukaryotic cells that plays a critical role in processes such as cytoskeleton organization, intracellular vesicular trafficking, secretion, cell motility, regulation of ion channels and nuclear signalling pathways. The enzymes responsible for the synthesis of PtdIns(4,5)P₂ are phosphatidylinositol phosphate kinases (PIPKs). The moss Physcomitrella patens contains two PIPKs, PpPIPK1 and PpPIPK2. To study their physiological role, both genes were disrupted by targeted homologous recombination and as a result mutant plants with lower PtdIns(4,5)P₂ levels were obtained. A strong phenotype for pipk1, but not for pipk2 single knockout lines, was obtained. The pipk1 knockout lines were impaired in rhizoid and caulonemal cell elongation, whereas pipk1‐2 double knockout lines showed dramatic defects in protonemal and gametophore morphology manifested by the absence of rapidly elongating caulonemal cells in the protonemal tissue, leafy gametophores with very short rhizoids, and loss of sporophyte production. pipk1 complemented by overexpression of PpPIPK1 fully restored the wild‐type phenotype whereas overexpression of the inactive PpPIPK1E885A did not. Overexpression of PpPIPK2 in the pipk1‐2 double knockout did not restore the wild‐type phenotype demonstrating that PpPIPK1 and PpPIPK2 are not functionally redundant. In vivo imaging of the cytoskeleton network revealed that the shortened caulonemal cells in the pipk1 mutants was the result of the absence of the apicobasal gradient of cortical F‐actin cables normally observed in wild‐type caulonemal cells. Our data indicate that both PpPIPKs play a crucial role in the development of the moss P. patens, and particularly in the regulation of tip growth.     

我国真菌传线状小麦花叶病毒病病原初步鉴定为小麦黄花叶病毒(WYMV)

由禾谷多粘菌（Ｐｏｌｙｍｙｘａｇｒａｍｉｎｉｓ）传播的线状小麦花叶病毒有两种,一种是加拿大首先报道的小麦梭条斑花叶病毒（ＷＳＳＭＶ）,另一种是日本报道的小麦黄花叶病毒（ＷＹＭＶ）。这两种病毒粒子形态以及血清学性质非常相似,但核酸序列存在一定差异。经反转录聚合酶链反应（ＲＴＰＣＲ）和单链构象多态性分析（ＳＳＣＰ）,明确我国广泛发生的禾谷多粘菌传线状小麦花叶病毒都是小麦黄花叶病毒,但供试的８个分离物ＲＮＡ１和ＲＮＡ２序列存在差异,无一彼此完全相同     

Construction of a pTOC-T vector using GST-ParE toxin for direct cloning and selection of PCR products

Using linker insertion mutations, we determined the most stable region of the parE gene which encodes a toxic protein (ParE) that inhibits growth of Escherichia coli. The toxicity of ParE was sustained until a 144bp linker was inserted into this region. We have developed a 3 T-overhang vector based on these characteristics of the GST-ParE toxin, and named pTOC-T. Because pTOC-T uses a post-segregational killing system, all transformants grown up on the plates can be considered as recombinants containing foreign DNA. pTOC-T not require X-Gal, IPTG or other substrates for selection. This T-vector using a positive selection system can be applied to various E. coli strains such as XL1-Blue, BL21, DH5, JM109, and JM110.Revisions requested 28 July 2004; Revisions received 7 September 2004     

Construction of a pTOC-T vector using GST-ParE toxin for direct cloning and selection of PCR products

Using linker insertion mutations, we determined the most stable region of the parE gene which encodes a toxic protein (ParE) that inhibits growth of Escherichia coli. The toxicity of ParE was sustained until a 144 bp linker was inserted into this region. We have developed a 3' T-overhang vector based on these characteristics of the GST-ParE toxin, and named pTOC-T. Because pTOC-T uses a post-segregational killing system, all transformants grown up on the plates can be considered as recombinants containing foreign DNA. pTOC-T not require X-Gal, IPTG or other substrates for selection. This T-vector using a positive selection system can be applied to various E. coli strains such as XL1-Blue, BL21, DH5alpha, JM109, and JM110.     

A new, rapid and simple procedure for direct cloning of PCR products into baculoviruses.

We propose a novel method for direct cloning of foreign genes into baculoviruses which avoids the use of bacterial transfer vectors. The foreign gene to be inserted is derived by PCR using appropriate primers each of which contains an additional 50 nt of baculovirus sequence for homologous recombination between the PCR-derived DNA and the baculovirus DNA, thus accomplishing insertion of the foreign gene into the baculovirus. The direct cloning of green fluorescent protein and beta-glucuronidase in different baculovirus loci is described. The method is simple and avoids the use of cumbersome techniques associated with enzymatic treatment and DNA purification.     

Detection of Helicobacter pylori in water by direct PCR

AIMS: This paper demonstrates a rapid, simple method for the detection of Helicobacter pylori in water that eliminates the need for recovery of cells or DNA extraction prior to PCR. METHODS AND RESULTS: Direct polymerase chain reaction (DPCR) with primers specific for H. pylori ureA (urease, subunit A) were used to detect H. pylori added to groundwater. DPCR also detected H. pylori in a naturally contaminated water sample. CONCLUSIONS: DPCR should provide an improved method to assess contamination of water by H. pylori. SIGNIFICANCE AND IMPACT OF THE STUDY: This simple, rapid method for detection of H. pylori in water will provide an improved means to investigate the possible role of water as a disease vector.     

Sebacinales are associates of the leafy liverwort Lophozia excisa in the southern maritime Antarctic

The leafy liverwort Lophozia excisa, which is colonised by basidiomycete fungi in other biomes and which evidence suggests may be colonised by mycorrhizal fungi in Antarctica, was sampled from Léonie Island in the southern maritime Antarctic (67°36′ S, 68°21′ W). Microscopic examination of plants indicated that fungal hyphae colonised 78% of the rhizoids of the liverwort, apparently by entering the tips of rhizoids prior to growing into their bases, where they formed hyphal coils. Extensive colonisation of stem medullary cells by hyphae was also observed. DNA was extracted from surface-sterilised liverwort tissues and sequenced following nested PCR, using the primer set ITS1F/TW14, followed by a second round of amplification using the ITSSeb3/TW13 primer set. Neighbour-joining analyses showed that the sequences obtained nested in Sebacinales clade B as a 100% supported sister group to Sebacinales sequences from the leafy liverworts Lophozia sudetica, L. incisa and Calypogeia muelleriana sampled from Europe. Direct PCR using the fungal specific primer set ITS1F/ITS4 similarly identified fungi belonging to Sebacinales clade B as the principal colonists of L. excisa tissues. These observations indicate the presence of a second mycothallus in Antarctica and support the previous suggestion that the Sebacinales has a wide geographical distribution.     

Simple cloning via direct transformation of PCR product (DNA Multimer) to Escherichia coli and Bacillus subtilis

We developed a general restriction enzyme-free and ligase-free method for subcloning up to three DNA fragments into any location of a plasmid. The DNA multimer generated by prolonged overlap extension PCR was directly transformed in Escherichia coli [e.g., TOP10, DH5α, JM109, and BL21(DE3)] and Bacillus subtilis for obtaining chimeric plasmids.     

Rapid amplification and cloning of Tn5 flanking fragments by inverse PCR

A simple approach is described to efficiently amplify DNA sequences flanking transposon Tn5 insertions. The method involves: (i) digestion with a restriction enzyme that cuts within Tn5; (ii) self-ligation under conditions favouring the production of monomeric circles; (iii) four parallel PCR reactions using primers designed to amplify left or right flanking sequences, and to distinguish target amplicons from non-specific products. This reveals the number of Tn5 insertions and the size of flanking genomic restriction fragments, without Southern blot analysis. The amplified product contains restriction sites that facilitate cohesive-end cloning. This rapid method is demonstrated using Tn5 and Tn5-Mob tagged DNA sequences involved in albicidin biosynthesis in Xanthomonas albilineans. It is generally applicable for efficient recovery of DNA sequences flanking transposon Tn5 derivatives in insertional mutagenesis studies.     

Detection and evaluation of non-recombinants in cDNA libraries by multiple cloning region PCR.

Bacteriophages that are routinely used in cDNA libraries do not require any biological selection for forming plaques. Thus parental non-recombinant phages are always found in variable proportions together with recombinant ones in all cDNA libraries. The presence of non-recombinants in significant proportions dilutes the abundance of rare cDNA species and makes library screening difficult. If the exact proportion of non-recombinants in a library were known, then one would screen proportionately more plaques to get a positive clone. In the absence of such information, screening is conventionally conducted on a number that is based on the titer of the library. We have devised a method using the flanking sequences from either side of the multiple cloning region (MCR) of all lambda phage vector derivatives as primers for PCR amplification. A non-recombinant phage produces a fragment equal to the size of the MCR, whereas a recombinant phage produces a fragment larger than the MCR, which is an MCR+ fragment. All cDNA libraries that we have studied show the presence of the MCR fragment (indicating non-recombinants) at variable proportions ranging between 6% and 36% of the total phages present. We also show that their presence negatively influences the retrieval of target cDNA sequences.     

Isolation and characterization ofVibrio vulnificus inhabiting the marine environment of the southwestern area of Taiwan

Vibrio vulnificus, a marine bacterium, is of concern in Taiwan because it causes wound infections and sepsis with a high mortality rate every year. To examine forV. vulnificus, 13 samples of seawater or oysters were collected from nine sites in Yunlin, Chiayi, and Tainan. Seventy-seven strains ofV. vulnificus were isolated from 11 samples. Among these environmental isolates, 72 (91%) were indole-positive, a characteristic of biotype 1. The remaining five strains although indole-negative, a characteristic previously found exclusively in biotype 2 strains, were all ornithine decarboxylase- and mannitol-positive, which has never been reported for biotype 2 strains. Based on the overall biochemical reactions obtained using a commercial identification system, these indole-negative strains appeared to be more like biotype 1. Fifty-seven ribotypes were identified among these isolates, indicating the great genetic divergence in this species. Of the 30 environmental isolates tested, 17 (56.7%) exhibited virulence comparable to the clinical isolates in the mouse, implying that a high proportion of theV. vulnificus strains in the marine environments might be pathogenic to humans.     

Ozone sensitivity in herbaceous species as assessed by direct and modulated chlorophyll fluorescence techniques

Seven plant species were exposed in open-top chambers to four levels of ozone (O₃) during two growing seasons and screened for treatment effects on the fast chlorophylla(Chl) fluorescence transient kinetics of dark-adapted leaves, and on the fluorescence signals obtained from the same leaves in illuminated steady-state. The aim was to identify the nature of O₃ effects on PSII, and to determine inter-specific differences. In dark-adapted leaves, O₃ caused a reduction in variable fluorescence (F_V : F₀), indicating an overall reduction in the efficiency of primary photochemistry. A large increase in excitation energy dissipation per active reaction centre (DI₀/RC) and a smaller increase in the trapping rate of excitons (TR₀/RC), showed that a fraction of the reaction centres was inactivated while the rest sustained full functionality. The magnitude of the effect increased in the order ofBromus erectusCentaurea jacea Trisetum flavescens Rumex obtusifolius Plantago lanceolataTrifolium pratense Knautia arvensis. The inter-specific variability in PSII responses could not be explained solely by specific differences in modelled O₃ uptake by the leaves. Visible leaf injury was not related to changes in fluorescence emission. In illuminated steady-state, O₃ sensitivity was most expressed in the change in quantum yield of photosynthetic electron transport (Φ_PSII). The ranking of species differed from the ranking obtained in dark-adapted leaves. These results suggest that the mechanistic basis for O₃ effects on PSII is similar in all species, but that inter-specific differences exist in the magnitude of change which cannot be explained solely by different O₃ uptake rates. The observed changes in fluorescence signals are not O₃-specific.     

Fungal diversity and functionality are driven by soil texture in Taylor Valley,Antarctica

The McMurdo Dry Valleys surface is mainly constituted from unconsolidated permafrost. Despite the combination of cold and dry conditions, transiently wetted soils close to lake edges are hotspots of intense biological activity, that can support the surrounding soil ecosystems in such extreme environments. These soils host simple microbial communities that allow easy characterization of the parameters determining microbial establishment and diversification. Soil samples were collected close to three different glacial lakes (Lake Fryxell, Lake Hoare and Lake Joyce) located along a longitudinal gradient from the lower to the upper Taylor Valley. Fungal diversity and functionality of sampled soils were studied through ITS1 metabarcoding sequencing. The correlation between the parameters describing fungal diversity (i.e. total richness, relative richness of dominant taxonomic and functional groups, and community composition) and the edaphic physicochemical parameters (i.e. pH, moisture, C, N, P, Na⁺, K⁺, Mg²⁺ and Ca²⁺, cation exchange capacity, and soil granulometry) was assessed. The fungal communities showed low richness (48 ± 32 OTUs per sample). Their composition was highly diversified even within different sites close to the same lake. The main parameters affecting the diversity and composition of fungal communities were soil texture, in turn influencing the retention of water and nutrients, and physicochemical properties. This is of particular concern for the survival of these communities, given the expected environmental changes due to global warming.