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Symbiotic penetrative association between a fungus and the roots of a vascular plant From Wikipedia, the free encyclopedia
An arbuscular mycorrhiza (AM) (plural mycorrhizae) is a type of mycorrhiza in which the symbiont fungus (AM fungi, or AMF) penetrates the cortical cells of the roots of a vascular plant forming arbuscules. Arbuscular mycorrhiza is a type of endomycorrhiza along with ericoid mycorrhiza and orchid mycorrhiza (not to be confused with ectomycorrhiza). They are characterized by the formation of unique tree-like structures, the arbuscules.[1] In addition, globular storage structures called vesicles are often encountered.
Arbuscular mycorrhizae are formed by fungi in the subphylum Glomeromycotina. This subphylum, along with the Mortierellomycotina, and Mucoromycotina, form the phylum Mucoromycota, a sister clade of the more well-known and diverse dikaryan fungi.[2]
AM fungi help plants to capture nutrients such as phosphorus, sulfur, nitrogen and micronutrients from the soil. It is believed that the development of the arbuscular mycorrhizal symbiosis played a crucial role in the initial colonisation of land by plants and in the evolution of the vascular plants.[3] It has been said that it is quicker to list the plants that do not form endomycorrhizae than those that do.[4] This symbiosis is a highly evolved mutualistic relationship found between fungi and plants, the most prevalent plant symbiosis known,[5] and AMF is found in 80% of vascular plant families in existence today.[6]
Previously this type of mycorrhizal associations were called 'Vesicular arbuscular mycorrhiza (VAM)', but since some members of these fungi do not produce any vesicles, such as the members of Gigasporaceae; the term has been changed to 'Arbuscular Mycorrhizae' to include them.[7][8]
Advances in research on mycorrhizal physiology and ecology since the 1970s have led to a greater understanding of the multiple roles of AMF in the ecosystem. An example is the important contribution of the glue-like protein glomalin to soil structure (see below). This knowledge is applicable to human endeavors of ecosystem management, ecosystem restoration, and agriculture.
Both paleobiological and molecular evidence indicate that AM is an ancient symbiosis that originated at least 460 million years ago. AM symbiosis is ubiquitous among land plants, which suggests that mycorrhizas were present in the early ancestors of extant land plants. This positive association with plants may have facilitated the development of land plants.[5]
The Rhynie chert of the lower Devonian has yielded fossils of the earliest land plants in which AM fungi have been observed.[10] The fossilized plants containing mycorrhizal fungi were preserved in silica.
The Early Devonian saw the development of terrestrial flora. Plants of the Rhynie chert from the Lower Devonian (400 m.yrs ago) were found to contain structures resembling vesicles and spores of present Glomus species. Colonized fossil roots have been observed in Aglaophyton major and Rhynia, which are ancient plants possessing characteristics of vascular plants and bryophytes with primitive protostelic rhizomes.[10]
Intraradical mycelium was observed in root intracellular spaces, and arbuscules were observed in the layer thin wall cells similar to palisade parenchyma. The fossil arbuscules appear very similar to those of existing AMF.[10] The cells containing arbuscules have thickened walls, which are also observed in extant colonized cells.
Mycorrhizas from the Miocene exhibit a vesicular morphology closely resembling that of present Glomerales. This conserved morphology may reflect the ready availability of nutrients provided by the plant hosts in both modern and Miocene mutualisms.[11] However, it can be argued that the efficacy of signaling processes is likely to have evolved since the Miocene, and this can not be detected in the fossil record. A finetuning of the signaling processes would improve coordination and nutrient exchange between symbionts while increasing the fitness of both the fungi and the plant symbionts.
The nature of the relationship between plants and the ancestors of arbuscular mycorrhizal fungi is contentious. Two hypotheses are:
Both saprotrophs and biotrophs were found in the Rhynie Chert, but there is little evidence to support either hypothesis.
There is some fossil evidence that suggests that the parasitic fungi did not kill the host cells immediately upon invasion, although a response to the invasion was observed in the host cells. This response may have evolved into the chemical signaling processes required for symbiosis.[10]
In both cases, the symbiotic plant-fungi interaction is thought to have evolved from a relationship in which the fungi was taking nutrients from the plant into a symbiotic relationship where the plant and fungi exchange nutrients.
The ancient plants did not have true roots. Strullu-Derrien and Strullu proposed the term 'Paramycorrhizae' for the mycorrhizae that infected the rhizome or shoot or thalli, and 'Eumycorrhizae' that infects true roots.[12][13][14] These structures were reported in both sporophytes and gametophytes of the early land plants.[13]
Increased interest in mycorrhizal symbiosis and the development of sophisticated molecular techniques has led to the rapid development of genetic evidence. Wang et al. (2010) investigated plant genes involved in communication with order Glomales fungal partners (DMI1, DMI3, IPD3).[15][16] These three genes could be sequenced from all major clades of modern land plants, including liverworts, the most basal group, and phylogeny of the three genes proved to agree with then current land plant phylogenies. This implies that mycorrhizal genes must have been present in the common ancestor of land plants, and that they must have been vertically inherited since plants colonized land.[15]
It was revealed that AM fungi have the bacterial type core enzyme (ribonuclease III) of the sRNA processing mechanism, probably by the process of horizontal gene transfer from a cyanobacterial ancestor, and possibly related to symbiosis,.[17] This finding of a genetic fossil inside AM fungi raises the possibility of an intimate relationship between AM fungi and cyanobacterial ancestors. A similar Geosiphon–Nostoc symbiosis was previously reported.[18]
Surprisingly, despite their long evolution as an underground partner of plant roots, whose environment is far from light or temperature fluctuation, AMF still have a conserved circadian clock whose fungal circadian oscillator (frq) is activated by the blue light, similar to the model circadian fungus Neurospora crassa.[19] The proven conservation of a circadian clock and output genes in R. irregulare opens the door to the study of circadian clocks in the fungal partner of AM symbiosis. The same research characterized the AMF frq gene,[19] which is the first frq gene identified outgroup of Dikarya, and suggests the frq gene evolution in the fungal kingdom is much older than previously thought.
The development of the AM fungi prior to root colonization, known as presymbiosis, consists of three stages: spore germination, hyphal growth, host recognition and appressorium formation.
Spores of the AM fungi are thick-walled multi-nucleate resting structures.[21] The germination of the spore does not depend on the plant, as spores have been germinated under experimental conditions in the absence of plants both in vitro and in soil. However, the rate of germination can be increased by host root exudates.[22] AM fungal spores germinate given suitable conditions of the soil matrix, temperature, carbon dioxide concentration, pH, and phosphorus concentration.[21]
The growth of AM hyphae through the soil is controlled by host root exudates known as strigolactones, and the soil phosphorus concentration.[23] Low-phosphorus concentrations in the soil increase hyphal growth and branching as well as induce plant exudation of compounds that control hyphal branching intensity.[22][24]
The branching of AM fungal hyphae grown in phosphorus media of 1 mM is significantly reduced, but the length of the germ tube and total hyphal growth were not affected. A concentration of 10 mM phosphorus inhibited both hyphal growth and branching. This phosphorus concentration occurs in natural soil conditions and could thus contribute to reduced mycorrhizal colonization.[24]
Root exudates from AMF host plants grown in a liquid medium with and without phosphorus have been shown to affect hyphal growth. Spores of Gigaspora margarita were grown in host plant exudates. Hyphae of fungi grown in the exudates from roots starved of phosphorus grew more and produced tertiary branches compared to those grown in exudates from plants given adequate phosphorus. When the growth-promoting root exudates were added in low concentration, the AM fungi produced scattered long branches. As the concentration of exudates was increased, the fungi produced more tightly clustered branches. At the highest-concentration arbuscules, the AMF structures of phosphorus exchange were formed.[24]
This chemotaxic fungal response to the host plants exudates is thought to increase the efficacy of host root colonization in low-phosphorus soils.[22] It is an adaptation for fungi to efficiently explore the soil in search of a suitable plant host.[24]
Further evidence that arbuscular mycorrhizal fungi exhibit host-specific chemotaxis, that enable hyphal growth toward the roots of a potential host plant: Spores of Glomus mosseae were separated from the roots of a host plant, nonhost plants, and dead host plant by a membrane permeable only to hyphae. In the treatment with the host plant, the fungi crossed the membrane and always emerged within 800 μm of the root, but not in the treatments with nonhost plants and dead plants.[25]
Molecular techniques have been used to understand the signaling pathways between arbuscular mycorrhizae and plant roots. In 2003 it was shown how the AM undergoes physiological changes in the presence of exudates from potential host plant roots, to colonize it. Host plant root exudates trigger and turn on AM fungal genes required for the respiration of spore carbon compounds. In experiments, transcription rate of 10 genes increased half-hour after exposure and at an even greater rate after 1 hour. after 4 hours exposure AM respond with morphological growth. Genes isolated from that time are involved in mitochondrial activity and enzyme production. The fungal respiration rate, measured by O2 consumption rate, increased by 30% 3 hours after exposure to root exudates, indicating that host plant root exudates stimulate AMF spore mitochondrial activity. It may be part of a fungal regulatory mechanism that conserves spore energy for efficient growth and the hyphal branching upon receiving signals from a potential host plant.[26]
When arbuscular mycorrhizal fungal hyphae encounter the root of a host plant, an appressorium or 'infection structure' forms on the root epidermis. From this structure hyphae can penetrate into the host's parenchyma cortex.[27] AM need no chemical signals from the plant to form the appressoria. AM fungi could form appressoria on the cell walls of "ghost" cells in which the protoplast had been removed to eliminate signaling between the fungi and the plant host. However, the hyphae did not further penetrate the cells and grow in toward the root cortex, which indicates that signaling between symbionts is required for further growth once appressoria are formed.[22]
Once inside the parenchyma, the fungus forms highly branched structures for nutrient exchange with the plant called arbuscules.[27] These are the distinguishing structures of arbuscular mycorrhizal fungus. Arbuscules are the sites of exchange for phosphorus, carbon, water, and other nutrients.[21] There are two forms: Paris type is characterized by the growth of hyphae from one cell to the next; and Arum type is characterized by the growth of hyphae in the space between plant cells.[28] The choice between Paris type and Arum type is primarily determined by the host plant family, although some families or species are capable of either type.[29][30]
The host plant exerts a control over the intercellular hyphal proliferation and arbuscule formation. There is a decondensation of the plant's chromatin, which indicates increased transcription of the plant's DNA in arbuscule-containing cells.[27] Major modifications are required in the plant host cell to accommodate the arbuscules. The vacuoles shrink and other cellular organelles proliferate. The plant cell cytoskeleton is reorganized around the arbuscules.
There are two other types of hyphae that originate from the colonized host plant root. Once colonization has occurred, short-lived runner hyphae grow from the plant root into the soil. These are the hyphae that take up phosphorus and micronutrients, which are conferred to the plant. AM fungal hyphae have a high surface-to-volume ratio, making their absorptive ability greater than that of plant roots.[31] AMF hyphae are also finer than roots and can enter into pores of the soil that are inaccessible to roots.[32] The fourth type of AMF hyphae grows from the roots and colonizes other host plant roots. The four types of hyphae are morphologically distinct.[21]
AM fungi are obligate symbionts. They have limited saprobic ability and depend on the plant for their carbon nutrition.[33] AM fungi take up the products of the plant host's photosynthesis as hexoses.
Carbon transfer from plant to fungi may occur through the arbuscules or intraradical hyphae.[34] Secondary synthesis from the hexoses by AM occurs in the intraradical mycelium. Inside the mycelium, hexose is converted to trehalose and glycogen. Trehalose and glycogen are carbon storage forms that can be rapidly synthesized and degraded and may buffer the intracellular sugar concentrations.[34] The intraradical hexose enters the oxidative pentose phosphate pathway, which produces pentose for nucleic acids.
Lipid biosynthesis also occurs in the intraradical mycelium. Lipids are then stored or exported to extraradical hyphae where they may be stored or metabolized. The breakdown of lipids into hexoses, known as gluconeogenesis, occurs in the extraradical mycelium.[34] Approximately 25% of the carbon translocated from the plant to the fungi is stored in the extraradical hyphae.[35] Up to 20% of the host plant's carbon may be transferred to the AM fungi.[34] This represents the host plant's considerable carbon investment in mycorrhizal network and contribution to the below-ground organic carbon pool.
Increasing the plant's carbon supply to the AM fungi increases uptake and transfer of phosphorus from fungi to plant.[36] Likewise, phosphorus uptake and transfer is lowered when the photosynthate supplied to the fungi is decreased. Species of AMF differ in their abilities to supply the plant with phosphorus.[37] In some cases, arbuscular mycorrhizae are poor symbionts, providing little phosphorus while taking relatively high amounts of carbon.[37]
The main benefit of mycorrhizas to plants has been attributed to increased uptake of nutrients, especially phosphorus. This may be due to increased surface area in contact with soil, increased movement of nutrients into mycorrhizae, a modified root environment, and increased storage.[32] Mycorrhizas can be much more efficient than plant roots at taking up phosphorus. Phosphorus travels to the root or via diffusion and hyphae reduce the distance required for diffusion, thus increasing uptake. The rate of phosphorus flowing into mycorrhizae can be up to six times that of the root hairs.[32] In some cases, the role of phosphorus uptake can be completely taken over by the mycorrhizal network, and all of the plant's phosphorus may be of hyphal origin.[37] Less is known about the role of nitrogen nutrition in the arbuscular mycorrhizal system and its impact on the symbiosis and community. While significant advances have been made in elucidating the mechanisms of this complex interaction, much investigation remains to be done.
Mycorrhizal activity increases the phosphorus concentration available in the rhizosphere. Mycorrhizae lower the root zone pH by selective uptake of NH4+ (ammonium-ions) and by releasing H+ ions. Decreased soil pH increases the solubility of phosphorus precipitates. The hyphal NH4+ uptake also increases the nitrogen flow to the plant as the soil's inner surfaces absorb ammonium and distribute it by diffusion.[35]
AM fungi have been regarded as asexual because they lack observable sexual structures.[38] However, homologs of 51 genes that function in meiosis, including seven meiosis-specific genes were found to be conserved in the genomes of several AMF species, suggesting that these supposedly ancient asexual fungi may be capable of undergoing conventional meiosis.[39] Furthermore, in Rhizophagus irregularis genetic exchange involving reciprocal recombination was found to occur in dikaryons between haploid genomes.[38]
Recent research has shown that AM fungi release an diffusional factor, known as the myc factor, which activates the nodulation factor's inducible gene MtEnod11. This is the same gene involved in establishing symbiosis with the nitrogen fixing, rhizobial bacteria (Kosuta et al. 2003). The factor was first identified by Fabienne Maillet and coworkers[40] in a groundbreaking work published in Nature, where they have extracted three hundred litre mycorrhized carrot roots and exudates from 40 million germinating spores of Rhizophagus irregularis and purified the active fraction. They demonstrated this active principle is lipo-chito-oligosaccharide in nature.
Recognition of Myc factors triggers the common symbiotic signaling pathway (CSSP) that eventually leads to plant's accommodation programme to provide hostage to the arbuscular mycorrhizae.
The Common Symbiotic Signaling Pathway (CSSP) is a Signaling cascade in plants that seen to be activated in both NOD-factor perception (for nodule forming Rhizobia), as well as found in MYC-factor perception that are released from Arbuscular mycorrhizal fungi. The pathway is distinguished from the pathogen recognition pathways, but may have some common receptors involved in both pathogen recognition as well as CSSP. A recent work[41] by Kevin Cope and colleagues shown that possibly other type of mycorrhizae may involve the CSSP components such as Myc-factor recognition.
The AMF colonization requires the following chain[42] of events that can be roughly divided into following steps -
Arbuscular mycorrhizal fungi are most frequent in plants growing on mineral soils, and are of extreme importance for plants growing in nutrient-deficient substrates such as in volcanic soil and sand dune environments. The populations of AM fungi is greatest in plant communities with high diversity such as tropical rainforests and temperate grasslands where they have many potential host plants and can take advantage of their ability to colonize a broad host range.[43] There is a lower incidence of mycorrhizal colonization in very arid or nutrient-rich soils. Mycorrhizas have been observed in aquatic habitats; however, waterlogged soils have been shown to decrease colonization in some species.[43] Arbuscular mycorrhizal fungi are found in 80% of plant species[44] and have been surveyed on all continents except Antarctica.[45][46] The biogeography of glomeromycota is influenced by dispersal limitation,[47] environmental factors such as climate,[45] soil series and soil pH,[46] soil nutrients[48] and plant community.[45][49] While evidence from 2000 suggests that AM fungi are not specialists on their host species,[50] studies as of 2002 have indicated that at least some fungi taxa are host specialists.[51] The ecology of Mucoromycotinian fungi, which form "fine root endophyte" arbuscular mycorrhizas is largely unknown.
The specificity, host range, and degree of colonization of mycorrhizal fungi are difficult to analyze in the field due to the complexity of interactions between the fungi within a root and within the system. There is no clear evidence to suggest that arbuscular mycorrhizal fungi exhibit specificity for colonization of potential AM host plant species as do fungal pathogens for their host plants.[43] This may be due to the opposite selective pressure involved.
In pathogenic relations, the host plant benefits from mutations that prevent colonization, whereas, in a mutualistic symbiotic relationship, the plant benefits from mutation that allow for colonization by AMF.[43] However, plant species differ in the extent and dependence on colonization by certain AM fungi, and some plants may be facultative mycotrophs, while others may be obligate mycotrophs.[43] Recently, mycorrhizal status has been linked to plant distributions,[52] with obligate mycorrhizal plants occupying warmer, drier habitats while facultative mycorrhizal plants occupy larger ranges of habitats.
The ability of the same AM fungi to colonize many species of plants has ecological implications. Plants of different species can be linked underground to a common mycelial network.[43] One plant may provide the photosynthate carbon for the establishment of the mycelial network that another plant of a different species can utilize for mineral uptake. This implies that arbuscular mycorrhizae are able to balance below-ground intra–and interspecific plant interactions.[43]
Since Glomeromycota fungi live inside plant roots, they can be influenced substantially by their plant host and in return affect plant communities as well. Plants can allocate up to 30% of their photosynthate carbon to AM fungi[53] and in return AM fungi can acquire up to 80% of plant phosphorus and nitrogen.[44] The diversity of AM fungal communities has been positively linked to plant diversity,[54] plant productivity[55] and herbivory.[56] Arbuscular mycorrhizal fungi can be influenced by small scale interactions with the local plant community. For example, the plant neighborhood around a focal plant can alter AM fungal communities[57] as can the order of plant establishment within sites.[58]
During invasions of plant species, the AM fungal community and biomass can be drastically altered. In the majority of cases AM fungal biomass and diversity decrease with invasions.[59][60][61] However, some mycotrophic plant species may actually increase AM fungal diversity during invasion.[62]
The mycorrhizal status of invasive plant species often varies between regions. For example, in the United Kingdom and central Europe recently invasive plants are more frequently obligately mycorrhizal than expected,[52][63] while invasive plants in California were found to be less frequently mycorrhizal than expected.[64]
All symbionts within a plant host interact, often in unpredictable ways. A 2010 meta-analysis indicated that plants colonized by both AM fungi and vertically transmitted endophytes often are larger than plants independently colonized by these symbionts.[65] However, this relationship is context-dependent as AM fungi can interact synergistically with fungal endophytes inhabiting the leaves of their host plant,[66][67] or antagonistically.[68][69][70] Similar ranges of interactions can occur between AM fungi and ectomycorrhizal fungi and dark septate endophytes.[71]
Arbuscular mycorrhizal fungi vary across many environmental gradients. Their tolerance to freezing and drying is known to shift between AM fungal taxa.[72] AM fungi become less prevalent and diverse at higher soil nutrient and moisture concentrations,[73] presumably because both plants allocate less carbon to AM fungi and AM fungi reallocate their resources to intraradical hyphae in these environmental conditions.[74] Over the long term, these environmental conditions can even create local adaptation between plant hosts, AM fungi and the local soil nutrient concentrations.[75] AM composition often becomes less diverse on mountain tops than at lower elevations, which is driven by the composition of plant species.[76]
AM fungi have been shown to improve plant tolerance to abiotic environmental factors such as salinity. They alleviate salt stress and benefit plant growth and productivity.[77]
The rhizosphere is the soil zone in the immediate vicinity of a root system.
Arbuscular mycorrhizal symbiosis affects the community and diversity of other organisms in the soil. This can be directly seen by the release of exudates, or indirectly by a change in the plant species and plant exudates type and amount.[78]
Mycorrhizae diversity has been shown to increase plant species diversity as the potential number of associations increases. Dominant arbuscular mycorrhizal fungi can prevent the invasion of non-mycorrhizal plants on land where they have established symbiosis and promote their mycorrhizal host.[79]
When rhizobium bacteria are present in the soil, mycorrhizal colonization is increased due to an increase in the concentration of chemical signals involved in the establishment of symbiosis (Xie et al. 2003). Molecules similar to Nod factors were isolated from AM fungi and were shown to induce MtEnod11, lateral root formation and enhance mycorrhization.[80] Effective mycorrhizal colonization can also increase the nodulations and symbiotic nitrogen fixation in mycorrhizal legumes.[35]
The extent of arbuscular mycorrhizal colonization and species affects the bacterial population in the rhizosphere.[81] Bacterial species differ in their abilities to compete for carbon compound root exudates. A change in the amount or composition of root exudates and fungal exudates due to the existing AM mycorrhizal colonization determines the diversity and abundance of the bacterial community in the rhizosphere.[78]
The influence of AM fungi on plant root and shoot growth may also have indirect effect on the rhizosphere bacteria. AMF contributes a substantial amount of carbon to the rhizosphere through the growth and degeneration of the hyphal network. There is also evidence to suggest that AM fungi may play an important role on mediating the plant species' specific effect on the bacterial composition of the rhizosphere.[78]
Global climate change is affecting AM fungal communities and interactions between AM fungi and their plant hosts. While it is generally accepted that interactions between organisms will affect their response to global climate change, we still lack the ability to predict the outcome of these interactions in future climates.[82] In recent meta-analyses, AM fungi were found to increase plant biomass under drought conditions and decrease plant biomass under simulated nitrogen deposition studies.[83][84] Arbuscular mycorrhizal fungi themselves have been shown to increase their biomass in response to elevated atmospheric CO2.[85]
Members of the mustard family (Brassicaceae), such as cabbage, cauliflower, canola, and crambe, do not establish arbuscular mycorrhizal fungi on their roots.[86]
In the past ten years there have been spectacular advances in molecular genetic technologies and tools. These advances allow microbial and mycorrhizal ecologists to ask new and exciting questions about the ecological and evolutionary roles of arbuscular mycorrhizal (AM) fungi as individuals, in communities and ecosystems. Genetic analyses of AM fungi have been used to explore the genetic structure of single spores using multilocus genotyping,[87] AM fungal diversity and adaptation across multiple grassland communities,[88] all the way up to a global investigation of AM fungal diversity, which greatly increased the described molecular diversity within the phylum Glomeromycota.[89]
All the recent advances in molecular genetics clearly permit the analysis of microbial communities at much finer and functional scales and potentially with more confidence than previous methods. The classical AM fungal identification method of spore extraction from soil and further spore morphological analysis[90] is fraught with complicating issues due to the various strategies and forms of AM fungi, e.g., lack of sporulation in certain species, seasonality, high unculturability, possible misidentification (human error), and new evidence of multi-nucleate spores[91] and high genetic variation within clonal AM species.[92] Because of these various problems, in the past researchers likely misrepresented the true composition of AM fungal communities present at any one point in time or place. Additionally, by following the traditional extraction, culture and microscopic identification methods, there is no way to determine active/functioning AM fungal populations, which are likely the most important when attempting to relate plant-AM symbiotic interactions and mechanisms to ecological or ecosystem function. This is especially true in the case of root colonization analyses, which can determine percentage of roots colonized by AM fungi. The major problem with this analysis is in field soils, which contain multiple species of AM fungi in association with a target plant at the same time (see Ecology of AM). The identification of the associated fungal symbionts is impossible without the use of molecular methods. Though genetic analysis of AM fungal communities has advanced a great deal in the past decade, the methodology is not yet completely refined. Below is an overview of the methods used in molecular genetic analyses of AM fungi, along with applications to research, future directions and some of their problems.
Genetic analyses of AM fungi from soil and root samples range in their applicability to answer ecological or phylogenetic questions. DNA analyses utilize various nuclear markers to describe AM fungi and represent different regions of the nuclear ribosomal operon (18S rRNA) found in all eukaryotic organisms. The DNA analysis of AM fungi using these markers began in the early 1990s[93] and are continuing to be developed today. The small subunit (SSU) rRNA gene, the internal transcribed spacer (ITS) gene, and the large subunit (LSU) rRNA gene are currently the most common DNA markers used. The SSU region has been used most frequently in ecological studies,[94] while the ITS and LSU regions have been predominantly used in taxonomic constructions of the phylum Glomeromycota.[95]
Real-time PCR or quantitative PCR (qPCR), is becoming a well-established method to quickly amplify and simultaneously quantify targeted AM fungal DNA from biological samples (plant roots or soils). Fairly recent developments in qPCR markers allow researchers to explore the relative abundance of AM fungal species within roots in greenhouse experiments as well as in the field to identify local AM fungal communities.
qPCR markers for arbuscular mycorrhizal fungi will consist of AM specific primers and fluorescently labeled hydrolysis probes. These AM specific primers (discussed above) can be chosen by the researcher and this decision is typically guided by the question at hand, resources available, and willingness to troubleshoot in the lab.
DNA microarray analysis is currently being used in AM fungal research to simultaneously measure the expression of many genes from target species or experimental samples. The most common tool or method is to use functional gene array (FGA) technology, a specialized microarray that contains probes for genes that are functionally important in microbial processes such as carbon, nitrogen or phosphorus cycling. FGAs have the ability to simultaneously examine many functional genes.[96] This technique is typically used for general analysis of functional microbial genes, but when complemented with genetic sequencing, inferences can be made about the connection between fungal community composition and microbial functionality.
Specific organismal chemical signatures can be used to detect biomass of more cryptic organisms, such as AM fungi or soil bacteria. Lipids, more specifically phospholipids and neutral lipids, contain fatty acids connected to a glycerol backbone. The fatty acid composition of organisms varies, and the proportions of specific fatty acids can be organism specific. For example, in AM fungi the proportion of the fatty acids, 16:1ω5 and 18:1ω7, in the phospholipid portion account for approximately 58% of total fatty acid composition.[97] The fatty acid, 16:1ω5 is the most commonly used acid to characterize AM fungi in soils and can be used as a strong indicator of mycelial biomass in soil sample.[97]
Neutral lipid fatty acid analysis of AM fungi is typically looked upon as a method to indicate energy storage, but most importantly, the ratio of NLFA (16:1ω5) to PLFA (16:1ω5) can potentially be used to indicate nutritional status of AM fungi in soils. Energy is mainly stored in AM fungi as neutral lipids in storage structures like spores and vesicles. Because of this NLFA correlates quite well with the number of spores in a given volume of soil.[97] The ratio of NLFA concentration to PLFA concentration (active mycelia) can then give the proportion of carbon allocated to storage structures (spores, measured as NLFA).
Problems with lipid fatty acid analyses include the incomplete specificity of fatty acids to AM fungi, the species- or genera-specific variation in fatty acid composition can complicate analysis in systems with multiple AM fungal species (e.g. field soil), the high background levels of certain fatty acid concentration in soils, and that phospholipids are correlated to an organism's membrane area, and the surface to volume ratio can vary widely between organisms such as bacteria and fungi.[98] More work must be done to identify the efficacy of this method in field soils with many genera and species of AM fungi to discern the methods ability to discriminate between many varying fatty acid compositions.
One prospect for future analysis of AM fungi is the use of stable isotope probes. Stable isotope probing (SIP) is a technique that can be used to determine the active metabolic function of individual taxa within a complex system of microbes. This level of specificity, linking microbial function and phylogenetics, has not been achieved previously in microbial ecology. This method can also be used independently of classical culture methods in microbial ecology, allowing for in situ analysis of functional microbes. Application of sequencing of single nucleus from spores of AM fungi has also been developed recently and also circumvents the need of culture methods.[99]
SIP, more explicitly DNA/RNA-based SIP, uses stable-isotope enriched substrates, such as 13C, 15N, or H218O, and then analyzes the 'labeled' markers using species specific DNA or RNA markers.[100] The analysis of labeled DNA is performed by separating unlabeled and labeled DNA on a cesium chloride gradient formed in an ultra centrifuge.[101] Because all microbial organisms are capable of importing water into their cells, the use of H218O stable isotope probing is a very exciting new method that can shed light on questions microbial ecologists and biologists have struggled with answering for years, in particular, what are the active microbial organisms in my system? The H218O, or heavy water method will target all organisms that are actively growing, and induce little influence on growth itself. This would be especially true with most greenhouse experiments with arbuscular mycorrhizas because plants must be watered anyway, and water does not directly select for organisms with specific metabolic pathways,[101] as would happen when using 13C and15N.
Little has been done with this method in arbuscular mycorrhizal experiments, but if proven to work in a controlled experiment, and with further refinement of DNA/RNA fungal community analyses techniques, this may be a viable option to very specifically determine the actively growing portion of AM fungal species across growing seasons, with different plant hosts or treatments, and in the face of climate change.
sRNAs have been reported to take crucial role in the crosstalk between host and symbiont.[102] sRNAs processing mechanism is thus, important for understanding AM symbiosis. It seems that AM fungi have their unique features to have bacterial type core enzyme as well as the large number of Argonaute proteins in their sRNA processing system (or RNAi system).[17] sRNA and sRNA processing mechanism research is also exciting topic to understand AM fungi symbiosis.
Disturbance of native plant communities in desertification-threatened areas is often followed by degradation of physical and biological soil properties, soil structure, nutrient availability, and organic matter. When restoring disturbed land, it is essential to replace not only the above ground vegetation but also biological and physical soil properties.[103]
A relatively new approach to restoring land is to inoculate soil with AM fungi when reintroducing vegetation in ecological restoration projects (phytoremediation). It has enabled host plants to establish themselves on degraded soil and improve soil quality and health.[104] Soils' quality parameters were significantly improved long-term when a mixture of indigenous arbuscular mycorrhizal fungi species was introduced compared to noninoculated soil and soil inoculated with a single exotic species of AM fungi.[103] The benefits were increased plant growth, increased phosphorus uptake[105] and soil nitrogen content, higher soil organic matter content, and soil aggregation, attributed to higher legume nodulation in the presence of AM fungi, better water infiltration, and soil aeration due to soil aggregation.[103] Native strains of AM fungi enhance the extraction of heavy metal(s) from the polluted soils and make the soil healthy and suitable for crop production.[106]
Many modern agronomic practices are disruptive to mycorrhizal symbiosis. There is great potential for low-input agriculture to manage the system in a way that promotes mycorrhizal symbiosis.
Conventional agriculture practices, such as tillage, heavy fertilizers and fungicides, poor crop rotations, and selection for plants that survive these conditions, hinder the ability of plants to form symbiosis with arbuscular mycorrhizal fungi.
Most agricultural crops can perform better and are more productive when well-colonized by AM fungi. AM symbiosis increases the phosphorus and micronutrient uptake and growth of their plant host (George et al. 1992).
Management of AM fungi is especially important for organic and low-input agriculture systems where soil phosphorus is, in general, low, although all agroecosystems can benefit by promoting arbuscular mycorrhizae establishment.
Some crops that are poor at seeking out nutrients in the soil are very dependent on AM fungi for phosphorus uptake. For example, flax, which has poor chemotaxic ability, is highly dependent on AM-mediated phosphorus uptake at low and intermediate soil phosphorus concentrations (Thingstrup et al. 1998).
Proper management of AMF in the agroecosystems can improve the quality of the soil and the productivity of the land. Agricultural practices such as reduced tillage, low phosphorus fertilizer usage, and perennialized cropping systems promote functional mycorrhizal symbiosis.
Tillage reduces the inoculation potential of the soil and the efficacy of mycorrhizaes by disrupting the extraradical hyphal network (Miller et al. 1995, McGonigle & Miller 1999, Mozafar et al. 2000).
By breaking apart the soil macro structure, the hyphal network is rendered non-infective (Miller et al. 1995, McGonigle & Miller 1999). The disruption of the hyphal network decreases the absorptive abilities of the mycorrhizae because the surface area spanned by the hyphae is greatly reduced. This, in turn, lowers the phosphorus input to the plants that are connected to the hyphal network (Figure 3, McGonigle & Miller 1999).
In reduced-tillage system, heavy phosphorus fertilizer input may not be required as compared to heavy-tillage systems. This is due to the increase in mycorrhizal network, which allows mycorrhizae to provide the plant with sufficient phosphorus (Miller et al. 1995).
The benefits of AMF are greatest in systems where inputs are low. Heavy usage of phosphorus fertilizer can inhibit mycorrhizal colonization and growth.
As the soil's phosphorus levels available to the plants increases, the amount of phosphorus also increases in the plant's tissues, and carbon drain on the plant by the AM fungi symbiosis become non-beneficial to the plant (Grant 2005).
A decrease in mycorrhizal colonization due to high soil-phosphorus levels can lead to plant deficiencies in other micronutrients that have mycorrhizal-mediated uptake such as copper (Timmer & Leyden 1980).
Cover crops are grown in the fall, winter, and spring, covering the soil during periods when it would commonly be left without a cover of growing plants.
Mycorrhizal cover crops can be used to improve the mycorrhizal inoculum potential and hyphal network (Kabir and Koide 2000, Boswell et al.1998, Sorensen et al. 2005).
Since AM fungi are biotrophic, they are dependent on plants for the growth of their hyphal networks. Growing a cover crop extends the time for AM growth into the autumn, winter, and spring. Promotion of hyphal growth creates a more extensive hyphal network. The mycorrhizal colonization increase found in cover crops systems may be largely attributed to an increase in the extraradical hyphal network that can colonize the roots of the new crop (Boswell et al. 1998). The extraradical mycelia are able to survive the winter, providing rapid spring colonization and early season symbiosis (McGonigle and Miller 1999). This early symbiosis allows plants to tap into the well-established hyphal network and be supplied with adequate phosphorus nutrition during early growth, which greatly improves the crop yield.
Restoration of native AM fungi increases the success of ecological restoration projects and the rapidity of soil recovery.[103] AM fungi enhance soil aggregate stability by the production of extraradical hyphae and a soil protein known as glomalin.
Glomalin-related soil proteins (GRSP) have been identified using a monoclonal antibody (Mab32B11) raised against crushed AMF spores. It is defined by its extraction conditions and reaction with the antibody Mab32B11.
There is other circumstantial evidence to show that glomalin is of AM fungal origin. When AM fungi are eliminated from soil through incubation of soil without host plants, the concentration of GRSP declines. A similar decline in GRSP has also been observed in incubated soils from forested, afforested, and agricultural land[108] and grasslands treated with fungicide.[109]
Glomalin is hypothesized to improve soil aggregate water stability and decrease soil erosion. A strong correlation has been found between GRSP and soil aggregate water stability in a wide variety of soils where organic material is the main binding agent, although the mechanism is not known.[109] The protein glomalin has not yet been isolated and described, and the link between glomalin, GRSP, and arbuscular mycorrhizal fungi is not yet clear.[109]
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