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1. Abyssal deposit feeders are secondary consumers of detritus and rely on nutrition derived from microbial communities in their guts

   https://doi.org/10.1038/s41598-021-91927-4  

   Romero-Romero, Sonia ; Miller, Elizabeth C. ; Black, Jesse A. ; Popp, Brian N. ; Drazen, Jeffrey C. ( December 2021 , Scientific Reports)

   null (Ed.)

   Abstract Trophic ecology of detrital-based food webs is still poorly understood. Abyssal plains depend entirely on detritus and are among the most understudied ecosystems, with deposit feeders dominating megafaunal communities. We used compound-specific stable isotope ratios of amino acids (CSIA-AA) to estimate the trophic position of three abundant species of deposit feeders collected from the abyssal plain of the Northeast Pacific (Station M; ~ 4000 m depth), and compared it to the trophic position of their gut contents and the surrounding sediments. Our results suggest that detritus forms the base of the food web and gut contents of deposit feeders have a trophic position consistent with primary consumers and are largely composed of a living biomass of heterotrophic prokaryotes. Subsequently, deposit feeders are a trophic level above their gut contents making them secondary consumers of detritus on the abyssal plain. Based on δ 13 C values of essential amino acids, we found that gut contents of deposit feeders are distinct from the surrounding surface detritus and form a unique food source, which was assimilated by the deposit feeders primarily in periods of low food supply. Overall, our results show that the guts of deposit feeders constitute hotspots of organic matter on the abyssal plain that occupy one trophic level above detritus, increasing the food-chain length in this detritus-based ecosystem. 

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2. Zooplankton trophic structure and ecosystem productivity

   https://doi.org/10.3354/meps14077  

   Décima, M ( June 2022 , Marine Ecology Progress Series)

   The number of trophic steps within a plankton food web plays an important role in determining the energy available to support higher-level consumers by affecting trophic transfer efficiency (TE): fewer steps can enhance TE by decreasing respiration and predation losses. In this study, trophic structure within the zooplankton community was investigated using stable isotopes in size-fractionated mesozooplankton, and related to 2 biomass proxies related to TE: the normalized biomass size spectra (NBSS) and the ratio of zooplankton:phytoplankton biomass (log 10 (zoo:phyto)). Four regions were compared: the California Current Ecosystem (CCE—most productive), the Equatorial Pacific (EqP), the Costa Rica Dome (CRD) and the North Pacific Subtropical Gyre (NPSG—least productive). Compound-specific isotope analysis of amino acids confirmed large differences (~3‰) in the isotopic baseline among ecosystems. EqP and NPSG had low and distinct source δ 15 N values, while CRD/CCE had high and overlapping values. Trophic differences indicated that the CCE had the lowest number (0) of trophic differences within the 4 zooplankton size classes; NPSG and EqP had the highest number (3), and CRD was intermediate (1). NBSS slopes confirmed the CCE and NPSG as extremes and statistically different from each other. TE patterns estimated from log 10 (zoo:phyto) suggested EqP was the least efficient, while the other 3 ecosystems (despite large ranges in zooplankton and phytoplankton biomass) had similar TEs. The inverse relationship between food chain length and system productivity, a paradigm originally formulated for microbial food webs, holds for the mesozooplankton assemblage at the productivity extremes. 

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3. Meta‐analysis of primary producer amino acid δ 15 N values and their influence on trophic position estimation

   https://doi.org/10.1111/2041-210X.13678  

   Ramirez, Matthew D. ; Besser, Alexi C. ; Newsome, Seth D. ; McMahon, Kelton W. ( August 2021 , Methods in Ecology and Evolution)

   Compound‐specific stable isotope analysis of individual amino acids (CSIA‐AA) has emerged as a transformative approach to estimate consumer trophic positions (TP_CSIA) that are internally indexed to primary producer nitrogen isotope baselines. Central to accurate TP_CSIAestimation is an understanding of beta (β) values—the differences between trophic and source AA δ¹⁵N values in the primary producers at the base of a consumers’ food web. Growing evidence suggests higher taxonomic and tissue‐specificβvalue variability than typically appreciated.

   This meta‐analysis fulfils a pressing need to comprehensively evaluate relevant sources ofβvalue variability and its contribution to TP_CSIAuncertainty. We first synthesized all published primary producer AA δ¹⁵N data to investigate ecologically relevant sources of variability (e.g. taxonomy, tissue type, habitat type, mode of photosynthesis). We then reviewed the biogeochemical mechanisms underpinning AA δ¹⁵N andβvalue variability. Lastly, we evaluated the sensitivity of TP_CSIAestimates to uncertainty in meanβ_Glx‐Phevalues and Glx‐Phe trophic discrimination factors (TDF_Glx‐Phe).

   We show that variation inβ_Glx‐Phevalues is two times greater than previously considered, with degree of vascularization, not habitat type (terrestrial vs. aquatic), providing the greatest source of variability (vascular autotroph = −6.6 ± 3.4‰; non‐vascular autotroph = +3.3 ± 1.8‰). Within vascular plants, tissue type secondarily contributed toβ_Glx‐Phevalue variability, but we found no clear distinction among C₃, C₄and CAM plantβ_Glx‐Phevalues. Notably, we found that vascular plantβ_Glx‐Lysvalues (+2.5 ± 1.6‰) are considerably less variable thanβ_Glx‐Phevalues, making Lys a useful AA tracer of primary production sources in terrestrial systems. Our multi‐trophic level sensitivity analyses demonstrate that TP_CSIAestimates are highly sensitive to changes in bothβ_Glx‐Pheand TDF_Glx‐Phevalues but that the relative influence ofβvalues dissipates at higher trophic levels.

   Our results highlight that primary producerβvalues are integral to accurate trophic position estimation. We outline four key recommendations for identifying, constraining and accounting forβvalue variability to improve TP_CSIAestimation accuracy and precision moving forward. We must ultimately expand libraries of primary producer AA δ¹⁵N values to better understand the mechanistic drivers ofβvalue variation.

    

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4. Intraspecific variation and energy channel coupling within a Chilean kelp forest

   https://doi.org/10.1002/ecy.3198  

   Elliott Smith, E ; Harrod, C ; Docmac, F ; Newsome, S. ( October 2020 , Ecology)

   Winemiller, KO. (Ed.)

   The widespread importance of variable types of primary production, or energy channels, to consumer communities has become increasingly apparent. However, the mechanisms underlying this “multichannel” feeding remain poorly understood, especially for aquatic ecosystems that pose unique logistical constraints given the diversity of potential energy channels. Here, we use bulk tissue isotopic analysis along with carbon isotope (δ13C) analysis of individual amino acids to characterize the relative contribution of pelagic and benthic energy sources to a kelp forest consumer community in northern Chile. We measured bulk tissue δ13C and δ15N for >120 samples; of these we analyzed δ13C values of six essential amino acids (EAA) from nine primary producer groups (n = 41) and 11 representative nearshore consumer taxa (n = 56). Using EAA δ13C data, we employed linear discriminant analysis (LDA) to assess how distinct EAA δ13C values were between local pelagic (phytoplankton/particulate organic matter), and benthic (kelps, red algae, and green algae) endmembers. With this model, we were able to correctly classify nearly 90% of producer samples to their original groupings, a significant improvement on traditional bulk isotopic analysis. With this EAA isotopic library, we then generated probability distributions for the most important sources of production for each individual consumer and species using a bootstrap‐resampling LDA approach. We found evidence for multichannel feeding within the community at the species level. Invertebrates tended to focus on either pelagic or benthic energy, deriving 13–67% of their EAA from pelagic sources. In contrast, mobile (fish) taxa at higher trophic levels used more equal proportions of each channel, ranging from 19% to 47% pelagically derived energy. Within a taxon, multichannel feeding was a result of specialization among individuals in energy channel usage, with 37 of 56 individual consumers estimated to derive >80% of their EAA from a single channel. Our study reveals how a cutting‐edge isotopic technique can characterize the dynamics of energy flow in coastal food webs, a topic that has historically been difficult to address. More broadly, our work provides a mechanism as to how multichannel feeding may occur in nearshore communities, and we suggest this pattern be investigated in additional ecosystems. 

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5. Stable isotope fingerprinting traces essential amino acid assimilation and multichannel feeding in a vertebrate consumer

   https://doi.org/10.1111/2041-210X.13903  

   Manlick, Philip J. ; Newsome, Seth D. ( June 2022 , Methods in Ecology and Evolution)

   Animals often consume resources from multiple energy channels, thereby connecting food webs and driving trophic structure. Such ‘multichannel feeding’ can dictate ecosystem function and stability, but tools to quantify this process are lacking. Stable isotope ‘fingerprints’ are unique patterns in essential amino acid (EAA) δ¹³C values that vary consistently between energy channels like primary production and detritus, and they have emerged as a tool to trace energy flow in wild systems. Because animals cannot synthesize EAAs de novo and must acquire them from dietary proteins, ecologists often assume δ¹³C fingerprints travel through food webs unaltered. Numerous studies have used this approach to quantify energy flow and multichannel feeding in animals, but δ¹³C fingerprinting has never been experimentally tested in a vertebrate consumer.

   We tested the efficacy of δ¹³C fingerprinting using captive deer micePeromyscus maniculatusraised on diets containing bacterial, fungal and plant protein, as well as a combination of all three sources. We measured the transfer of δ¹³C fingerprints from diet to consumer liver, muscle and bone collagen, and we used linear discriminant analysis (LDA) and isotopic mixing models to estimate dietary proportions compared to known contributions. Lastly, we tested the use of published δ¹³C source fingerprints previously used to estimate energy flow and multichannel feeding by consumers.

   We found that EAA δ¹³C values exhibit significant isotopic (i.e. trophic) fractionation between consumer tissues and diets. Nevertheless, LDA revealed that δ¹³C fingerprints are consistently routed and assimilated into consumer tissues, regardless of isotopic incorporation rate. Isotopic mixing models accurately estimated the proportional diets of consumers, but all models overestimated plant‐based protein contributions, likely due to the digestive efficiencies of protein sources. Lastly, we found that δ¹³C source fingerprints from published literature can lead to erroneous diet reconstruction.

   We show that δ¹³C fingerprints accurately measure energy flow to vertebrate consumers across tissues with different isotopic incorporation rates, thereby enabling the estimation of multichannel feeding at various temporal scales. Our findings illustrate the power of δ¹³C fingerprinting for quantifying food web dynamics, but also reveal that careful selection of dietary source data is critical to the accuracy of this emerging technique.

    

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