Manuel Kleiner scite author profile

Microbial community structure can be analyzed by quantifying cell numbers or by quantifying biomass for individual populations. Methods for quantifying cell numbers are already available (e.g., fluorescence in situ hybridization, 16S rRNA gene amplicon sequencing), yet high-throughput methods for assessing community structure in terms of biomass are lacking. Here we present metaproteomics-based methods for assessing microbial community structure using protein abundance as a measure for biomass contributions of individual populations. We optimize the accuracy and sensitivity of the method using artificially assembled microbial communities and show that it is less prone to some of the biases found in sequencing-based methods. We apply the method to communities from two different environments, microbial mats from two alkaline soda lakes, and saliva from multiple individuals. We show that assessment of species biomass contributions adds an important dimension to the analysis of microbial community structure.

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Metaproteomics of a gutless marine worm and its symbiotic microbial community reveal unusual pathways for carbon and energy use

Kleiner

Wentrup

Lott

et al. 2012

Proc. Natl. Acad. Sci. U.S.A.

187

251

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Low nutrient and energy availability has led to the evolution of numerous strategies for overcoming these limitations, of which symbiotic associations represent a key mechanism. Particularly striking are the associations between chemosynthetic bacteria and marine animals that thrive in nutrient-poor environments such as the deep sea because the symbionts allow their hosts to grow on inorganic energy and carbon sources such as sulfide and CO 2 . Remarkably little is known about the physiological strategies that enable chemosynthetic symbioses to colonize oligotrophic environments. In this study, we used metaproteomics and metabolomics to investigate the intricate network of metabolic interactions in the chemosynthetic association between Olavius algarvensis, a gutless marine worm, and its bacterial symbionts. We propose previously undescribed pathways for coping with energy and nutrient limitation, some of which may be widespread in both freeliving and symbiotic bacteria. These pathways include (i) a pathway for symbiont assimilation of the host waste products acetate, propionate, succinate and malate; (ii) the potential use of carbon monoxide as an energy source, a substrate previously not known to play a role in marine invertebrate symbioses; (iii) the potential use of hydrogen as an energy source; (iv) the strong expression of high-affinity uptake transporters; and (v) as yet undescribed energy-efficient steps in CO 2 fixation and sulfate reduction. The high expression of proteins involved in pathways for energy and carbon uptake and conservation in the O. algarvensis symbiosis indicates that the oligotrophic nature of its environment exerted a strong selective pressure in shaping these associations.3-hydroxypropionate bi-cycle | Calvin cycle | proton-translocating pyrophosphatase | pyrophosphate dependent phosphofructokinase | metagenomics G rowth in nutrient-limited environments presents numerous challenges to organisms. Symbiotic and syntrophic relationships have evolved as particularly successful strategies for coping with these challenges. Such nutritional symbioses are widespread in nature and, for example, have enabled plants to colonize nitrogen-poor soils and animals to thrive on food sources that lack essential amino acids and vitamins (1). Chemosynthetic symbioses, discovered only 35 years ago at hydrothermal vents in the deep sea, revolutionized our understanding of nutritional associations, because these symbioses enable animals to live on inorganic energy and carbon sources such as sulfide and CO 2 (2, 3). The chemosynthetic symbionts use the energy obtained from oxidizing reduced inorganic compounds such as sulfide to fix CO 2 , ultimately providing their hosts with organic carbon compounds. Chemosynthetic symbioses thus are able to thrive in habitats where organic carbon sources are rare, such as the deep sea, and the symbionts often are so efficient at providing nutrition that many hosts have reduced their digestive systems (4).The marine oligochaete Olavius algarvensis is a particularly extre...

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Evaluation of methods to purify virus-like particles for metagenomic sequencing of intestinal viromes

2015

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BackgroundViruses are a significant component of the intestinal microbiota in mammals. In recent years, advances in sequencing technologies and data analysis techniques have enabled detailed metagenomic studies investigating intestinal viromes (collections of bacteriophage and eukaryotic viral nucleic acids) and their potential contributions to the ecology of the microbiota. An important component of virome studies is the isolation and purification of virus-like particles (VLPs) from intestinal contents or feces. Several methods have been applied to isolate VLPs from intestinal samples, yet to our knowledge, the efficiency and reproducibility between methods have not been explored. A rigorous evaluation of methods for VLP purification is critical as many studies begin to move from descriptive analyses of virus diversity to studies striving to quantitatively compare viral abundances across many samples. Therefore, reproducible VLP purification methods which allow for high sample throughput are needed. Here we compared and evaluated four methods for VLP purification using artificial intestinal microbiota samples of known bacterial and viral composition.ResultsWe compared the following four methods of VLP purification from fecal samples: (i) filtration + DNase, (ii) dithiothreitol treatment + filtration + DNase, (iii) filtration + DNase + PEG precipitation and (iv) filtration + DNase + CsCl density gradient centrifugation. Three of the four tested methods worked well for VLP purification. We observed several differences between methods related to the removal efficiency of bacterial and host DNAs and biases against specific phages. In particular the CsCl density gradient centrifugation method, which is frequently used for VLP purification, was most efficient in removing host derived DNA, but also showed strong discrimination against specific phages and showed a lower reproducibility of quantitative results.ConclusionsBased on our data we recommend the use of methods (i) or (ii) for large scale studies when quantitative comparison of viral abundances across samples is required. The CsCl density gradient centrifugation method, while being excellently suited to achieve highly purified samples, in our opinion, should be used with caution when performing quantitative studies.Electronic supplementary materialThe online version of this article (doi:10.1186/s12864-014-1207-4) contains supplementary material, which is available to authorized users.

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Manuel Kleiner

Assessing species biomass contributions in microbial communities via metaproteomics

Metaproteomics of a gutless marine worm and its symbiotic microbial community reveal unusual pathways for carbon and energy use

Evaluation of methods to purify virus-like particles for metagenomic sequencing of intestinal viromes

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