Figures
Abstract
A cross-transplant experiment between estuarine water and seawater was conducted to examine the response of bacterial metabolic activity to riverine dissolved organic carbon (DOC) input under virus-rich and virus-free conditions, as well as to exogenous viruses. Riverine DOC input increased bacterial production significantly, but not bacterial respiration (BR) because of its high lability. The bioavailable riverine DOC influenced bulk bacterial respiration in two contrasting ways; it enhanced the bulk BR by stimulating bacterial growth, but simultaneously reduced the cell-specific BR due to its high lability. As a result, there was little stimulation of the bulk BR by riverine DOC. This might be partly responsible for lower CO2 degassing fluxes in estuaries receiving high sewage-DOC that is highly labile. Viruses restricted microbial decomposition of riverine DOC dramatically by repressing the growth of metabolically active bacteria. Bacterial carbon demand in the presence of viruses only accounted for 7–12% of that in the absence of viruses. Consequently, a large fraction of riverine DOC was likely transported offshore to the shelf. In addition, marine bacteria and estuarine bacteria responded distinctly to exogenous viruses. Marine viruses were able to infect estuarine bacteria, but not as efficiently as estuarine viruses, while estuarine viruses infected marine bacteria as efficiently as marine viruses. We speculate that the rapid changes in the viral community due to freshwater input destroyed the existing bacteria-virus relationship, which would change the bacterial community composition and affect the bacterial metabolic activity and carbon cycling in this estuary.
Citation: Xu J, Sun M, Shi Z, Harrison PJ, Liu H (2014) Response of Bacterial Metabolic Activity to Riverine Dissolved Organic Carbon and Exogenous Viruses in Estuarine and Coastal Waters: Implications for CO2 Emission. PLoS ONE 9(7): e102490. https://doi.org/10.1371/journal.pone.0102490
Editor: Douglas Andrew Campbell, Mount Allison University, Canada
Received: April 29, 2014; Accepted: June 19, 2014; Published: July 18, 2014
Copyright: © 2014 Xu et al. This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
Data Availability: The authors confirm that all data underlying the findings are fully available without restriction. All relevant data are within the paper.
Funding: Financial support for this research was provided by the Hundred Talented Program Startup Fund (Y35L041001) by South China Sea Institute of Oceanology, the Key Project of National Natural Science Fundation of China (No. 91128212) and the University Grants Council of Hong Kong AoE project (AoE/P-04/04-4-II). The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.
Competing interests: The authors have declared that no competing interests exist.
Introduction
Estuaries are in general a significant source of CO2 to the atmosphere, where CO2 efflux is estimated to be 0.25±0.25 Pg C y−1 at the global scale [1]. Low-latitude estuarine/coastal waters receive approximately two-thirds of the terrestrial organic carbon (OC) and have higher microbial decomposition rates due to higher temperatures [2]–[5]. Hence, it is speculated that more CO2 is degassing in lower latitude estuarine and coastal waters [1].
The Pearl River is subtropical and the second largest river in China, with an annual average freshwater discharge of 10,524 m3 s−1, which was calculated by Yin et al. [6] from Zhao [7]. About 80% of the discharge occurs in the wet season (April–September). High dissolved organic carbon (DOC) concentrations up to 473 µmol C L−1 occur in the Pearl River estuary, most of which originates from sewage [8]. However, the CO2 degassing flux is reported to be 6.92 mol C m2 y−1 in the entire Pearl River estuary [9], much lower than that (36.5–182.5 mol C m2 y−1) for the European estuaries [4], [10]. Similarly, low CO2 flux (only 8.1 mol C m2 y−1) has also been documented in the Hoogly estuary (NE India) that receives a huge amount (∼400 million tons yearly) of sewage [11]. One explanation for the surprisingly lower CO2 flux in these low-latitude estuaries is due to the large freshwater discharge and short residence time of the discharged water [12], [13]. To date, the underlying mechanism for the lower CO2 flux remains unknown.
The riverine DOC is primarily mineralized by heterotrophic bacteria that produce a significant amount of new biomass from DOC and transform DOC into inorganic carbon [14]–[16]. High terrestrial organic carbon input exerts a great influence on bacterial metabolism and community composition [17], [18]. Prior studies suggest that the lability of DOC plays a key role in regulating bacterial respiration rates [19]. Cell-specific bacterial respiration increases sharply in response to the decreasing quality of DOC since a larger percentage of energy is used for maintenance processes to safeguard metabolic flexibility at the cost of energetic efficiency [19], [20]. A recent study indicates that bacteria grown on sewage-derived DOC have high production and low respiration rates, while those on marine-derived DOC at have high respiration rates [21]. Hence, the lability of DOC could potentially affect CO2 degassing fluxes in high DOC estuaries.
In recent years, it has been recognized that viruses play an important role in regulating bacterial metabolic activities [22]–[24]. Bacterial production is reported to be reduced by up to 50% due to viral lysis [25]. However, little attention has been paid to interactions between bacteria and indigenous viruses and the effect of viruses on microbial decomposition of riverine DOC in estuaries, which may be important in understanding the fate of terrestrial organic carbon in the ocean. To our knowledge, only few studies have been conducted which suggested that the bacterial response to different sources of viruses may vary [26]–[28]. Therefore, a study on response of bacterial metabolic processes to riverine DOC and exogenous viruses is needed to determine the reasons for the lower CO2 degassing fluxes in the Pearl River estuary. A cross-transplant experiment of estuarine water and seawater was conducted to examine the response of bacterial metabolic activity to riverine DOC input under virus-rich and virus-free conditions. This study will increase our understanding of the role of bacteria in influencing riverine organic carbon cycling in estuarine waters.
Materials and Methods
No specific permissions were required for sampling at stations PM7 and NM3 in Hong Kong waters. We confirmed that the field studies did not involve endangered or protected species at these two stations. Seawater samples were taken from 1 m depth in August (wet summer season) 2013 at two contrasting coastal sites, a relatively pristine coastal station (PM7) with no influence from sewage or freshwater discharge, and a eutrophic estuarine station near the Pearl River (NM3) (Fig. 1). The water depths of PM7 and NM3 were 17 and 15 m, respectively. Samples for nutrients, dissolved organic carbon (DOC), and bacterial and viral abundance were taken.
These 2 stations are the same as the Environmental Protection Department of Hong Kong monitoring stations. The water depths for NM3 and PM7 are 15 and 17
Experimental set-up
Water samples were passed through a 1 µm polycarbonate membrane and the filtrate was used as the bacterial inoculum. Virus-rich water was obtained by filtration of water samples through a 0.1 µm cartridge. Relatively virus-free water was prepared by filtration of the 0.1 µm filtrate through a 100 kDa cutoff polysulfone cartridge (Millipore) using tangential flow ultra-filtration. About 600 ml of the bacterial inoculum was mixed with 5.4 L of virus-rich and relatively virus-free water from each station in acid-washed and Milli-Q rinsed polycarbonate carboys and distributed to triplicate glass bottles (1 L) to obtain eight treatments (Fig. 2) as follows: 1) estuarine bacteria + virus-rich estuarine water (Be+Ve); 2) estuarine bacteria + virus-free estuarine water (Be-Ve); 3) estuarine bacteria + virus-rich seawater (Be+Vs); 4) estuarine bacteria + virus-free seawater (Be-Vs); 5) marine bacteria + virus-rich estuarine water (Bs+Ve); 6) marine bacteria + virus-free estuarine water (Bs-Ve); 7) marine bacteria + virus-rich seawater (Bs+Vs) and; 8) marine bacteria + virus-free seawater (Bs-Vs).
Bs and Be denote marine and estuarine bacteria, respectively. Vs and Ve denote marine and estuarine viruses, respectively.
Samples were incubated in the dark for 24 h. Running seawater was used to maintain the surface in situ temperature. Samples for nutrients, bacterial abundance (BA), bacterial production (BP), bacterial respiration (BR), viral abundance (VA) were taken at the beginning and end of the incubations. DOC samples were taken at the beginning of the incubation.
Nutrients and DOC concentrations
Nutrient concentrations (NO3,, NH4, PO4 and SiO4) were determined colorimetrically with a SKALAR autoanalyser following the protocols described by Strickland and Parsons [29] and Grasshoff et al. [30]. Dissolved inorganic nitrogen (DIN) was the sum of NO3,
and NH4. Samples for DOC were filtered through a 0.2 µm acetate cellulose membrane and analyzed with a high temperature combustion method using a Shimadzu TOC-5000 analyzer [31].
Bacterial and viral abundance, bacterial production, respiration and cell size
Samples for bacterial and viral abundance were taken in micro-centrifuge tubes, fixed with buffered paraformaldehyde (final concentration 0.5%), and then stored at −80°C until analysis by a flow cytometer (Becton-Dickinson FACSCalibur). Bacterial and viral abundance was determined according to the methods described by Marie et al. [32], [33] and Xu et al. [24], respectively. Bacteria were determined on a plot of green fluorescence vs. side scatter (SSC), which also provided information on the relative DNA content and cell size by the means of SYB-green fluorescence side scatter, respectively. The values for relative DNA content and cell size were calibrated with 1 µm sized beads.
The measurement of bacterial production (BP) and bacterial respiration (BR) was described previously [24]. BP was measured using 3H-leucine following the JGOFS protocol [31] and the final concentration of 3H-leucine was 35 nM. BP was calculated with the empirical conversion factor of 3 kg C mol leucine−1 [34]. Dissolved oxygen for bacterial respiration was titrated using an automated titration apparatus (716 DMS Titrino Metrohm) [35]. BR was presented in carbon units assuming that the respiratory quotient was 1 [36].
Bulk BP was calculated using the following equation:where BPi and BPf are bacterial production (µg C L−1 h−1) measured at the beginning and the end of the experiment, Δt is the time interval between the beginning and the end of the experiment.
The cell-specific BP (sBP) and BR (sBR) were calculated according to the following equations, respectively:where Ai and Af are the initial and final abundance of bacteria, respectively.
The growth rates of bacteria and viruses were calculated using the following equation:where Ai and Af are the initial and final abundance of bacteria or viruses, respectively. Δt is the time interval between the beginning and the end of the experiment.
Bacterial growth efficiency was calculated using the following equation:
Statistical analyses
Statistical analyses were performed using SPSS software. A parametric ANOVA analysis with an LSD (least square difference) multiple comparison technique was conducted to determine any significant difference between treatments (p<0.05). The error bars represent the standard error from triplicates for each treatment.
Results
Surface salinity (22.40) at estuarine station (NM3) was much lower than that (28.64) at coastal station (PM7) (Table 1). Nutrient and DOC concentrations were high at NM3 and low at PM7. However, bacterial and viral abundance (2.45×109 cells L−1 and 2.57×1010 particles L−1, respectively) at PM7 was higher than those (4.28×108 cells L−1 and 9.40×109 particles L−1, respectively) at NM3 (Table 1).
For the bioassay experiments with estuarine bacteria, viral abundance was the highest (1.95×1010 particles L−1) in the Be+Vs treatment, moderate (1.00×1010 particles L−1) in the Be+Ve treatment and the lowest (∼2.20×109 particles L−1) in the Be-Ve and Be-Vs treatments (Fig. 3). The abundance ratio of viruses to bacteria followed the pattern of viral abundance. Bacterial growth rates differed significantly among the four treatments, with low growth rates (2.9 and 2.6 d−1) in the virus-rich treatment (i.e. Be+Ve and Be+Vs) and high (3.7 and 5.3 d−1) in the virus-free treatment (i.e. Be-Ve and Be-Vs). The relative cell size and DNA content of bacteria followed the pattern of bacterial growth rate (Fig. 3). Bacterial production (535 and 118 µg L−1 d−1) and cell-specific bacterial production (134 and 136 fg cell−1 d−1) in the virus-free conditions (i.e. Be-Ve and Be-Vs) was significantly higher than the counterpart (42.7 and 40.6 µg L−1 d−1) and (79.3 and 106 fg cell−1 d−1) in the virus-rich conditions (i.e. Be+Ve and Be+Vs), respectively. Bacterial production did not differ significantly between the Be+Ve and Be+Vs treatment, while the cell-specific bacterial production in the Be+Vs treatment was significantly higher than that in the Be+Ve treatment. Similarly, bacterial respiration and cell-specific bacterial respiration followed the same patterns as bacterial production and cell-specific bacterial production, respectively (Fig. 4).
Bacterial growth rate, relative cell size, and relative DNA content at the end of the incubation among eight treatments: 1) estuarine bacteria + virus-rich estuarine water (Be+Ve); 2) estuarine bacteria + virus-free estuarine water (Be-Ve); 3) estuarine bacteria + virus-rich seawater (Be+Vs); 4) estuarine bacteria + virus-free seawater (Be-Vs); 5) seawater bacteria + virus-rich estuarine water (Bs+Ve); 6) seawater bacteria + virus-free estuarine water (Bs-Ve); 7) seawater bacteria + virus-rich seawater (Bs+Vs); 8) seawater bacteria + virus-free seawater (Bs-Vs). Vertical bars indicate ± 1SE and n = 3. Different letters (a, b, c, d) denote that the treatment was significantly different (p<0.05) and the same letters denote that the treatment was not significantly different (p>0.05).
Error bars indicate ± 1SE and n = 3. Different letters (a, b, c, d) denote that the treatment was significantly different (p<0.05) and the same letters denote that the treatment was not significantly different (p>0.05). See Fig. 3 for treatment abbreviations.
For the bioassay experiments with marine bacteria, viral abundance was the highest (2.10×1010 particles L−1) in the Bs+Vs treatment, moderate (1.33×1010 particles L−1) in the Bs+Ve treatment and the lowest (∼3.30×109 particles L−1) in the Bs-Ve and Bs-Vs treatments (Fig. 3). Bacterial growth rates differed significantly among four treatments, being low (1.1 and 1.0 d−1) in the autochthonous DOC treatment (i.e. Bs+Vs and Bs-Vs) and high (1.7 and 3.2 d−1) in the riverine DOC treatment (i.e. Bs+Ve and Bs-Ve). The relative cell size and DNA content of bacteria showed the same pattern (Fig. 3). Bacterial production (586 and 39.1 µg L−1 d−1) and cell-specific bacterial production (178 and 84.4 fg cell−1 d−1) in the virus-free conditions (i.e. Bs-Ve and Be-Vs) was significantly higher than the counterpart (56.0 and 19.5 µg L−1 d−1) and (65.4 and 34.5 fg cell−1 d−1) in the virus-rich conditions (i.e. Bs+Ve and Bs+Vs), respectively. Bacterial production and cell-specific bacterial production in the Bs+Ve treatment were significantly higher than those in the Bs+Vs treatment. Bacterial respiration (783 and 209 µg L−1 d−1) in the virus-free conditions (i.e. Bs-Ve and Bs-Vs) was significantly higher than that (110 and 112 µg L−1 d−1) in the virus-rich conditions (i.e. Bs+Ve and Bs+Vs), while bacterial respiration did not differ significantly between the Bs+Ve and Bs+Vs treatment. The cell-specific bacterial respiration (239 and 438 fg cell−1 d−1) in the virus-free conditions (i.e. Bs-Ve and Bs-Vs) was significantly higher than that (129 and 197 fg cell−1 d−1) in the virus-rich conditions (i.e. Bs+Ve and Bs+Vs) (Fig. 4).
For the bioassay experiments with marine bacteria, bacterial production and cell-specific bacterial production on the riverine DOC were significantly higher than those on the autochthonous coastal DOC (Stn PM7), irrespective of the presence and absence of viruses. Bacterial respiration on the riverine DOC was significantly higher than that on the autochthonous DOC in the virus-free conditions, but not in the virus-rich conditions. In contrast, the cell-specific bacterial respiration (129 and 239 fg cell−1 d−1) on the riverine DOC was significantly lower than that (197 and 438 fg cell−1 d−1) on autochthonous DOC, irrespective of the presence or absence of viruses. Bacterial growth efficiency (0.33 and 0.43) on the riverine DOC was significantly higher than that (0.15 and 0.17) on autochthonous DOC, irrespective of the presence or absence of viruses (Fig.4).
Discussion
Response of bacterial metabolic activity to riverine DOC input
The effects of DOC on bacterial metabolic activity are often assessed in the presence of viruses, which might bias the bacterial response to DOC supply alone [37] and underestimate bioavailability of DOC. In this study, a comparison of the bacterial response to riverine DOC between the presence or absence of viruses provided insight into the bioavailability of riverine DOC and the role of viruses in regulating carbon cycling in the Pearl River estuary.
Our results showed that bacterial metabolic activity responded significantly to the riverine DOC input irrespective of the presence or absence of viruses. Generally, bacterial production, cell-specific BP, growth rate, relative cell size and DNA content were significantly higher in the riverine DOC treatments (e.g. Bs+Ve and Bs-Ve) than the counterpart in the autothchonous coastal DOC treatments (e.g. Bs+Vs and Bs-Vs), respectively. These results suggested that riverine DOC was highly bioavailable and efficiently utilized, which favored the growth of large and metabolically active marine bacteria, especially under virus-free conditions. However, in the presence of viruses, the increased DOC utilization was mitigated considerably by viral lyses, since the large and metabolically active bacteria may have been preferentially killed by viruses [38] and less competitive bacterial species that were resistant to viral infection survived [39], [40]. In addition, the viral shunt is partly responsible for low bacterial production in the presence of viruses [41]. It is estimated that up to 50% of bacterial mortality is due to viral lyses in marine environments [22], [25]. A significant correlation between bacterial production and the relative DNA content or cell size (Fig. 5) further confirmed that viruses played a major role in regulating bacterial production. The stimulation of bacterial production by riverine DOC in the presence of viruses implied that the addition of bioavailable DOC might, to some extent, weaken viral control of bacterial production by improving the capability of the metabolically active bacteria to resist viral lysis. This finding was consistent with previous reports [42], [43].
In response to riverine DOC input, the bulk bacterial respiration was enhanced significantly in the absence of viruses, but not in the presence of viruses, which was contradictory with previous reports that viruses enhanced the role of bacteria as oxidizers of organic matter and producers of CO2 by stimulating bacterial respiration [26]. Viral infection has been reported to enhance BR likely due to the decomposition of the viral lysate with an energetic cost [44]. Interestingly, the cell-specific bacterial respiration in the riverine DOC treatments (i.e. Bs+Ve and Bs-Ve) was significantly lower than that in the autochthonous coastal DOC treatments (Bs+Vs and Bs-Vs) irrespective of the presence or absence of viruses, which was the opposite pattern for the cell-specific bacterial production. The cell-specific bacterial respiration has been found to be sensitive to changes in substrates, which increases sharply with the deceasing quality and quantity of the substrates [20], [24]. The high cell-specific bacterial production and low cell-specific bacterial respiration in the riverine DOC treatment further corroborated that riverine DOC was highly labile, resulting in higher bacterial growth efficiency. An early study showed that sewage effluents with high concentrations of carbohydrates and amino acids, which are among the most labile fraction of the bulk organic matter [45], [46], were the major sources (32–54%) of riverine DOC in the Pearl River estuary [8]. Our observations are in agreement with the finding from our previous sewage-seawater cross-transplant experiment that sewage effluents enhanced bacterial production, but not bacterial respiration, resulting in high bacterial growth efficiency [21]. The bioavailable riverine DOC input influenced the bulk bacterial respiration in two contrasting ways; it enhanced the bulk BR by stimulating bacterial growth and reduced the cell-specific BR due to its high lability. Riverine DOC input altered the partitioning between production and respiration within the natural bacterial community, with a larger proportion of carbon used for biomass synthesis and less for maintenance. The high supply of riverine DOC exposed bacteria to labile DOC in the Pearl River estuary with repaid discharge and a short residence time. As a result, there was little stimulation of the bulk BR by riverine DOC. This might partly explain the lower CO2 emission in some estuaries that receive a large amount of riverine DOC with a high percentage of sewage-derived DOC. The relatively low bacterial production in the presence of viruses was more likely due to the repression of the metabolically active bacteria, rather than the viral shunt, since the viral shunt would increase bacterial respiration [26], [47].
Viral infection dramatically decreased bacterial carbon demand. Bacterial carbon demand ( = BP+BR) in the presence of viruses only accounted for 7–12% of that in the absence of viruses. The bioavailability of riverine DOC in the presence of viruses was greatly underestimated, since bacterial production was primarily regulated by viruses, rather than DOC [24]. In conventional microbial decomposition experiments, the biodegradable DOC is estimated as the difference between the DOC at the beginning and end of the incubation that could last for several days or up to one month. In this case, the estimated bioavailability of DOC is likely biased because a fraction of the bacterial biomass is returned to the DOC pool as semi-labile or recalcitrant DOC via the viral shunt [48], which might be substantial during a long-term incubation.
Response of bacterial metabolic activity to exogenous viruses
Shifts in the viral community composition are observed along a salinity gradient in estuaries [49], as well as viral infection rates [50]. To date, little attention has been paid to the composition and metabolic response of the natural bacterial assemblage to varying sources of viruses in estuaries [27]. In our study, bacterial mortality induced by exogenous viruses was assessed through a cross-transplant experiment of estuarine water and seawater. The relative cell size, DNA content, and cell-specific bacterial production in the Be+Vs treatment were significantly lower than that in the Be-Vs treatment, suggesting that marine viruses were able to repress the metabolically active estuarine bacteria. However, the cell-specific bacterial production in the Be+Ve treatment was significantly lower than that in the Be+Vs treatment, despite the high DOC availability in the Be+Ve treatment, implying that marine viruses were able to infect estuarine bacteria, but not as efficiently as estuarine viruses. This was inconsistent with a previous report that marine viruses may not be able to infect freshwater bacteria [27]. In contrast, a 2.7-fold difference in the cell-specific bacterial production for marine bacteria between in virus-free (Bs-Ve) and virus-rich (Bs+Ve) estuarine water was similar to the difference (2.4-fold) between in virus-free (Bs-Vs) and virus-rich (Bs+Vs) seawater. It revealed that estuarine viruses were able to efficiently infect marine bacteria. The same finding has been reported by Bonilla-Findji et al. [27]. The rapid changes in the viral community induced by freshwater input into estuaries might alter the existing relationship between bacteria and viruses, leading to changes in bacterial metabolic activity and community composition along a salinity gradient in estuarine environments, in addition to the salinity effect [51], [52]. As the capability of utilizing the various DOC component varies with the type of microorganism [53], the effect of changes in the bacterial community composition and bacterial metabolic activity induced by exogenous viruses on the carbon cycle in estuaries should not be ignored. Further studies are needed to confirm the interaction of bacteria and exogenous viruses.
Evaluation of the Experimental Approach
Recent studies suggest that salinity may be an important factor regulating virus-host interactions [52], [54]. In this study, estuarine water in the middle section of the Pearl River estuary served as the riverine DOC source instead of freshwater in the upper section of the estuary, in order to reduce the effect of low salinity on the bacterial metabolic activity in our experiments. Our earlier study has shown that large bacteria typically captured on a 1 µm polycarbonate membrane filter were negligible when the bacterial inoculum was prepared [21]. The empirical conversion factor of 3.0 kg C mol leucine−1 was adopted to calculate bacterial production and we cannot rule out the possibility that BP for bacteria grown on autochthonous DOC was overestimated, since DOC at coastal station PM7 was at the relatively low level and less labile. The DNA content is a useful proxy for bacterial activity [55]. The significant correlation between cell-specific bacterial production and relative DNA content (Fig. 5) indicated that the estimation of BP based on the commonly used empirical conversion factor was valid.
Conclusions
Riverine DOC input increased bacterial production significantly, but not bacterial respiration because of its high lability. The bioavailable riverine DOC input influenced the bulk bacterial respiration in two contrasting ways; it enhanced the bulk BR by stimulating bacterial growth and reduced the cell-specific BR due to its high lability. As a result, there was little stimulation of the bulk BR by riverine DOC. The lability of riverine DOC might be partly responsible for lower CO2 degassing fluxes in some DOC-rich estuaries. Viruses reduced bacterial carbon demand dramatically by repressing the growth of metabolically active bacteria, which eventually restricted microbial decomposition of riverine DOC. Bacterial carbon demand in the presence of viruses only accounted for 7–12% of that in the absence of viruses. Hence, a significant fraction of riverine DOC was transported offshore to the shelf and slope ocean.
Author Contributions
Conceived and designed the experiments: JX PH HL. Performed the experiments: JX MS ZS. Analyzed the data: JX. Contributed reagents/materials/analysis tools: JX MS ZS. Contributed to the writing of the manuscript: JX PH HL.
References
- 1. Cai WJ (2011) Estuarine and coastal ocean carbon paradox: CO2 sinks or sites of terrestrial carbon incineration? Annu Rev Mar Sci 3: 123–145.
- 2. Laws EA, Falkowski PG, Smith WO Jr, Ducklow H, McCarthy JJ (2000) Temperature effects on export production in the open ocean. Glob Biogeochem Cycles 14: 1231–1246.
- 3. Price PB, Swoers T (2004) Temperature dependence of metabolic rates for microbial growth, maintenance, and survival. Proc Natl Acad Sci U S A 101: 4631–4636.
- 4. Borges AV, Dellile B, Frankignoulle M (2005) Budgeting sinks and sources of CO2 in the coastal ocean: diversity of ecosystems counts. Geophys Res Lett 32: L14601.
- 5. Fuhrman JA, Steele JA, Hewson I, Schwalbach MS, Brown MV, et al. (2008) A latitudinal diversity gradient in planktonic marine bacteria. Proc Natl Acad Sci U S A 1005: 7774–7778.
- 6. Yin K, Qian PY, Chen JC, Hsieh DPH, Harrison PJ (2000) Dynamics of nutrients and phytoplankton biomass in the Pearl River estuary and adjacent waters of Hong Kong during summer: preliminary evidence for phosphorus and silicon limitation. Mar Ecol Prog Ser 194: 295–305.
- 7.
Zhao H (1990) Evolution of the Pearl River estuary. Ocean Press, Beijing (in Chinese).
- 8. He BY, Dai MH, Zhai WD, Wang LF, Wang KJ, et al. (2010) Distribution, degradation and dynamics of dissolved organic carbon and its major compound classes in the Pearl River estuary, China. Mar Chem 119: 52–64.
- 9. Guo X, Dai M, Zhai W, Cai WJ, Chen B (2009) CO2 flux and seasonal variability in a large subtropical estuarine system, the Pearl River estuary, China. J Geophys Res 114: G03013.
- 10. Zhai WD, Dai MH, Guo XH (2007) Carbonate system and CO2 degassing fluxes in the inner estuary of Changjiang (Yangtze) River, China. Mar Chem 107: 342–356.
- 11. Mukhopadhyay SK, Biswas H, De TK, Sen S, Jana TK (2002) Seasonal effects on the air-water carbon dioxide exchange in the Hooghly estuary, NE coast of Bay of Bengal, India. J Environ Monit 41: 549–552.
- 12. Shetye SR (1999) Propagation of tides in the Mandovi and Zuri estuaries. Sadhana 24: 5–16.
- 13. Sundar D, Shetye SR (2005) Tides in the Mandovi and Zuari estuaries, Goa, west coast of India. J Earth Syst Sci 114: 493–503.
- 14. Williams PJL (1981) Microbial contribution to overall marine plankton metabolism: direct measurement of respiration. Oceanologica Acta 4: 359–364.
- 15. Pomeroy LR, Wiebe WJ, Deibel D, Thompson JR, Rowe GT, et al. (1991) Bacterial responses to temperature and substrate concentration during the Newfoundland spring bloom. Mar Ecol Prog Ser 75: 143–159.
- 16.
Fuhrman JA (1992) Bacterioplankton roles in cycling of organic matter: the microbial food web, p 361–383. In Woodhead PGF (ed), Primary Productivity and Biogeochemical Cycles in the Sea, Plenum Press, New York.
- 17. Stepanauskas R, Leonardson L, Tranvik LJ (1999) Bioavailability of wetland-derived DON to freshwater and marine bacterioplankton. Limnol Oceanogr 44: 1477–1485.
- 18. Langenheder S, Kisand V, Lindström ES, Wikner J, Tranvik LJ (2004) Growth dynamics within bacterial communities in riverine and estuarine batch cultures. Aquat Microb Ecol 37: 137–148.
- 19. Carlson CA, del Giorgio PA, Herndl GJ (2007) Microbes and the dissipation of energy and respiration: from cells to ecosystems. Oceanography 20: 89–100.
- 20.
del Giorgio PA, Cole JJ (2000) Bacterial energetics and growth efficiency, p 289–325. In Kirchman KL (ed), Microbial ecology of the ocean, Wiley-Liss Inc., New York.
- 21. Xu J, Jing H, Kong L, Sun M, Harrison PJ, et al. (2013) Effect of seawater-sewage cross-transplants on bacterial metabolism and diversity. Microb Ecol 66: 60–72.
- 22. Bouvier T, del Giorgio PA (2007) Key role of selective virus-induced mortality in determining marine bacterioplankton composition. Environ Microbiol 9: 287–297.
- 23. Campbell B, Yu L, Heidelberg JF, Kirchman DL (2011) Activity of abundant and rare bacteria in a coastal ocean. Proc Nat Acad Sci U S A 108: 12776–12781.
- 24. Xu J, Jing H, Sun M, Harrison PJ, Liu H (2013) Regulation of bacterial metabolic activity by dissolved organic carbon and viruses. J Geophys Res Biogeosci 118: 1573–1583.
- 25. Fuhrman JA, Schwalbach M (2003) Viral influence on aquatic bacterial communities. Biol Bull 204: 192–195.
- 26. Bonilla-Findji O, Malits A, Lefèvre D, Rochelle-Newall E, Lemée R, et al. (2008) Viral effects on bacterial respiration, production and growth efficiency: Consistent trends in the Southern Ocean and the Mediterranean Sea. Deep-Sea Res II 55: 790–800.
- 27. Bonilla-Findji O, Rochelle-Newall E, Weinbauer MG, Pizay MD, Kerros ME, et al. (2009) Effect of seawater-freshwater cross-transplantations on viral dynamics and bacterial diversity and production. Aquat Microb Ecol 54: 1–11.
- 28. Rochelle-Newall EJ, Pizay MD, Middelburg JJ, Boschker HTS, Gattuso JP (2004) Degradation of riverine dissolved organic matter by seawater bacteria. Aquat Microb Ecol 37: 9–22.
- 29. Strickland JDH, Parsons TR (1968) Determination of reactive nitrate. In: A practical handbook of seawater analysis. Bull Fish Res Board Can167: 71–75.
- 30.
Grasshoff KM, Ehrhardt M, Kremling K (1983) Methods of seawater analysis. Weinheim, Verlag Chemie.
- 31.
Knap A, Michaels A, Close A, Ducklow H, Dickson A (1996) Protocols for the Joint Global Ocean Flux Study (JGOFS) core measurement, Rep. JGOFS Nr. 19, IOC Manual and Guide, No 29, UNESCO.
- 32. Marie D, Partensky F, Jacquet S, Vaulot D (1997) Enumeration and cell cycle analysis of natural populations of marine picoplankton by flow cytometry using the nucleic acid stain SYBR Green I. Appl Environ Microbiol. 63: 186–193.
- 33. Marie D, Brussaard CPD, Thyrhaug R, Bratbak G, Vaulot D (1999) Enumeration of marine viruses in culture and natural samples by flow cytometry. Appl Environ Microbiol 65: 45–52.
- 34. Pedrós-Alió C, Calderón-Paz J, Guixa-Boixereu N, Estrada M, Gasol JM (1999) Bacterioplankton and phytoplankton biomass and production during summer stratification in the northwestern Mediterranean Sea. Deep Sea Res I 46: 985–1019.
- 35. Outdot CR, Gerard R, Morin P, Gningue I (1988) Precise shipboard determination of dissolved oxygen (Winkler procedure) for productivity studies with a commercial system. Limnol Oceanogr 33: 146–150.
- 36. Hopkinson CS Jr (1985) Shallow-water benthic and pelagic metabolism: Evidence of heterotrophy in the nearshore Georgia Bight. Mar Biol 87: 19–32.
- 37. Zhang R, Weinbauer MG, Tam YK, Qian PY (2013) Response of bacterioplankton to a glucose gradient in the absence of lysis and grazing. FEMS Microbiol Ecol 85: 443–451.
- 38. Thingstad TF, Lignell R (1997) Theoretical models for the control of bacterial growth rate, abundance, diversity and carbon demand. Aquat Microb Ecol 13: 19–27.
- 39. Hewson I, Vargo GA, Fuhrman JA (2003) Bacterial diversity in shallow oligotrophic marine benthos and overlying waters: effects of virus infection, containment, and nutrient enrichment. Microb Ecol 46: 322–336.
- 40. Winter C, Smit A, Herndl GJ, Weinbauer MG (2005) Linking bacterial richness with viral abundance and prokaryotic activity. Limnol Oceanogr 50: 968–977.
- 41. Motegi C, Nagata T, Miki T, Weinbauer MG, Legendre L, et al. (2009) Viral control of bacterial growth efficiency in marine pelagic environments. Limnol Oceanor 54: 1901–1910.
- 42. Motegi C, Nagata T (2009) Addition of monomeric and polymeric organic substrates alleviates lytic pressure on bacterial communities in coastal seawaters. Aquat Microb Ecol 57: 343–350.
- 43. Zhang R, Weinbauer MG, Qian PY (2007) Viruses and flagellates sustain apparent richness and reduce biomass accumulation of bacterioplankton in coastal marine waters. Environ Microbiol 9: 3008–3018.
- 44. Middelboe M, Lyck PG (2002) Regeneration of dissolved organic matter by viral lysis in marine microbial communities. Aquat Microb Ecol 27: 187–194.
- 45. Benner R, Pakulski JD, McCarthy M, Hedges JI, Hatcher PG (1992) Bulk chemical characteristics of dissolved organic matter in the ocean. Science 255: 1561–1564.
- 46. Middelboe M, Borch NH, Kirchman DL (1995) Bacterial utilization of dissolved free amino acids, dissolved combined amino acids and ammonium in the Delaware Bay estuary: effects of carbon and nitrogen limitation. Mar Ecol Prog Ser 128: 109–120.
- 47. Eissler Y, Sahlsten E, Quiñones RA (2003) Effects of virus infection on respiration rates of marine phytoplankton and microplankton communities. Mar Ecol Prog Ser 262: 71–80.
- 48. Jiao N, Herndl GJ, Hansell DA, Benner R, Kattner G, et al. (2010) Microbial production of recalcitrant dissolved organic matter: long-term carbon storage in the global ocean. Nat Rev Microbiol 8: 593–599.
- 49. Wommack KE, Ravel J, Hill RT, Chun J, Clowell RR (1999) Population dynamics of Chesapeake Bay virioplankton: total-community analysis by pulse-field gel electrophoresis. Appl Environ Microbiol 65: 231–240.
- 50. Almeida MA, Cunda MA, Alcantara F (2001) Loss of estuarine bacteria by viral infection and predation in microcosm conditions. Microb Ecol 42: 562–571.
- 51. Lozupone CA, Knight R (2007) Global patterns in bacterial diversity. Proc Natl Acad Sci U S A 104: 11436–11440.
- 52. Combe M, Bouvier T, Pringault O, Rochelle-Newal E, Bouvier C, et al. (2013) Freshwater prokaryote and virus communities can adapt to a controlled increase in salinity through changes in their structure and interactions. Estuar Coast Shelf Sci 133: 58–66.
- 53. Carlson CA, Giovannoni SJ, Hansell DA, Goldberg SJ, Parsons R, et al. (2004) Interactions among dissolved organic carbon, microbial processes, and community structure in the mesopelagic zone of the northwestern Sargasso Sea. Limnol Oceanogr 49: 1073–1083.
- 54. Kukkaro P, Bamford DH (2009) Virus–Host interactions in environments with a wide range of ionic strengths. Environ Microbiol Reports 1: 71–77.
- 55. Jellet JF, Li WKW, Dickie PM, Boraie A, Kepkay PE (1996) Metabolic activity of bacterioplankton communities assessed by flow cytometry and single carbon substrate utilization. Mar Ecol Prog Ser 136: 213–225.