2.6. High-throughput sequencing and microbial diversity analysis

The purified amplicons were pooled in equimolar and paired-end sequenced on an Illumina MiSeq PE300 platform/NovaSeqPE250 platform (Illumina, San Diego, USA) according to the standard protocols by Majorbio Bio-Pharm Technology Co., Ltd. (Shanghai, China).

The raw bacterial 16S rRNA and Symbiodiniaceae ITS2 sequencing reads were demultiplexed, quality filtered by fastp version 0.20.0 (Chen et al., 2018), and merged by FLASH version 1.2.7 (Magoè and Salzberg, 2011) with the following criteria: (i) the 300 bp reads were truncated at any site receiving an average quality score of <20 over a 50 bp sliding window, and the truncated reads shorter than 50 bp and reads containing ambiguous characters were discarded; (ii) only overlapping sequences longer than 10 bp were assembled according to their overlapped sequence. The maximum mismatch ratio of the overlap region is 0.2. The reads that could not be assembled were discarded; (iii) samples were distinguished according to the barcode and primers, and the sequence direction was adjusted with exact barcode matching or a maximum of two nucleotide mismatch in primer matching.

Operational taxonomic units (OTUs) with a 97% similarity cutoff were clustered using the UPARSE version 7.1 (Edgar, 2013), and the chimeric sequences were identified and removed. The taxonomy of each OTU representative sequence was analyzed by RDP Classifier version 2.2 (Wang et al., 2007) according to the SILVA ribosomal RNA database and algal symbionts Genomic resource database (Shi et al., 2021), using a confidence threshold of 0.7. Alpha diversity index, including observed OTUs, and richness estimators, such as Ace, Chao, Shannon, and Simpson indices, were calculated based on the frequency of OTUs and genera in the assigned sequence collections after rare sequences were removed. The OTUs were analyzed by Student’s t-test to compare the difference of the abundance on the genus level.

3.6. Effect of Vibrio infection on the algal symbionts

The community of algal symbionts was also analyzed to assess the effects of Vibrio infection as shown in Figure 9. The community of algal symbionts was observed with the most components of Cladocopium sp. in coral holobionts and very few Breviolum sp. and Fugacium sp. in live stone and seawater. No significant difference in community abundance and diversity was observed among the groups in coral holobiont, which indicated the rare effect of Vibrio on the algal symbionts, and therefore verified that the phenomenon of bleaching might be caused by the bacterial infection reasoned by Vibrio and secondary disorder of bacterial community.

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FIGURE 9

Community component of algal symbionts in the coral culture system. The total genomic DNA from each group performed high-throughput sequencing using the primer pair of ITS-DINO and ITS2Rev2. The taxonomy of each OTU representative sequence was analyzed according to the algal symbionts’ genomic resource database and classified by ITS2 type.

4.2. Microbial shift and bacterial interaction behind Vibrio infection

In this article, the infection of V. fortis was designed as the only variable factor in coral health. The symptom development of coral bleaching and tissue lysis verified and strongly supported the hypothesis of “bacterial bleaching.” The findings in this study demonstrated that its infection also caused significant changes in the coral-associated microsystem, especially the increased abundance of opportunistic pathogenic bacteria, which might synergistically affect coral health.

Among the microbial community, the decreasing abundance of Bacillus belonging to phylum Firmicutes seems to be the most serious side effect caused by Vibrio infection (Figure 5). Bacillus had been widely accepted as the main antagonistic bacteria and used for biological control in agriculture (Jiang et al., 2018) and aquaculture (Wang et al., 2019), and recently reported as marine probiotics to increase coral resistance to bleaching (Rosado et al., 2019). Bacillus can produce secondary metabolites, including lipopeptides and polyketones with antibacterial, antiviral, or antitumor activities (Wu et al., 2019), and the quorum quenching (QQ) enzymes, such as AiiA (Dong et al., 2000) and YtnP (Sun et al., 2021), to degrade AHLs, inhibiting the biofilm formation and toxin release of AHLs/Lux-mediated pathogens including V. fortis that was known to contain an AHLs intermediated LuxM/LuxN QS pathway (Ding et al., 2014). The subsequent abnormal abundant Bacillus, B. circulans for instance, resulted from the simulated outbreaking of V. fortis when the inoculation of 10⁵ CFU/ml was far beyond the threshold of QS; therefore, it might further weaken the resistance of coral holobiont to the stress from pathogens (Satpute et al., 2010; Niu et al., 2014).

The increased abundance of Rhodococcus in phylum Actinobacteria might also be related to the decreasing abundance of Bacillus, because Rhodococcus sp. was reported with antibacterial activity against Bacillus substilis (Mahmoud and Kalendar, 2016). Among these, the most composition species, R. erythropolis, produces different types of QQ enzymes (Ryu et al., 2020) to recognize and degrade AHLs and could be used for biofouling control (Ergön-Can et al., 2017). The increasing abundance might be speculated to result from the self-regulation of the coral symbiotic microbiota after the sense of abnormally increased concentration of AHLs generated by the inoculated V. fortis.

The increasing abundance of the genera Ralstonia and Burkholderia–Caballeronia–Paraburkholderia in phylum Proteobacteria was probably eligible for the causal relationship of the declined abundance of Bacillus because of the less inhibition from the Bacillus-produced surfactin (Grady et al., 2019). However, the correlation between Ralstonia and Burkholderia–Caballeronia–Paraburkholderia of coral health is still unclear (Bernasconi et al., 2019). Reports are claiming that Ralstonia sp. is a known gram-negative phytopathogenic bacteria (Hayashi et al., 2019) and dental opportunistic pathogen (Tuttlebee et al., 2002), while the Burkholderia–Caballeronia–Paraburkholderia, which is mostly constituted by Paraburkholderia fungorum, is reported as a plant probiotic bacteria (Rahman et al., 2018) but still risky to human health (Tan et al., 2020).

In addition, considering that the planktonic bacteria in the water could flow into the gastrovascular cavity of coral along with the filter feeding, the significantly increased abundance of Thalassobius (also detected with higher abundance in bleaching coral but with no significant difference) and Tenacibaculum in water might also affect the coral health (Figure 7). Thalassobius belonging to the family Rhodobacteraceae has been reported as a microbial bioindicator enriched in the Stony Coral Tissue Loss Disease accompanied by Vibrio (Becker et al., 2021), and has been associated with invertebrate diseases (Roder et al., 2014), while the increased abundance of Tenacibaculum was also consistent with the findings from microbial community shift in the White syndrome-affected Echinopora lamellosa in aquaria (Smith et al., 2015).

Another unclassified genus belonging to the family Rhodobacteraceae and the genus Shimia was also detected in the planktonic bacterial community in water, though there was no significant difference observed yet. The indicator species in the coral hosts, family Rhodobacteraceae and genus Shimia, were observed to increase their relative abundance when corals are under stress (Casey et al., 2015; Pootakham et al., 2019) or with the emergence of Porites white patch syndrome accompanied with Vibrio (Séré et al., 2013). This phenomenon was verified in the later coral bleaching in the blank group caused by the deterioration of water quality 2 days after the experiments stopped (data not shown).

The virulence from the shift bacterial community of abundant opportunistic pathogens might not be the only reason for coral bleaching. The nutrients sources and waste products for coral holobiont are also a concern, which mainly come from the metabolism of symbiotic microbes such as carbon and nitrogen fixation (Gibbin et al., 2019) and the metabolic integration from algal symbionts (Sun et al., 2020), in such closed aquaria without extra exogenous nutrient sources. The shift in the bacterial community no doubt leads to an imbalance in the nutrient food chain in the coral holobiont (Raina et al., 2009); however, in this study, there is no direct relevance between the infection of V. fortis and the status of algal symbionts. The dominant population in the tested S. guttatus was Cladocopium sp., though with few relative abundances of other Symbiodiniaceae according to the reported ITS2 type (Yu et al., 2020), and no observation of Durusdinium sp., which was reported with stronger stress resistance (Sun et al., 2020); therefore, the findings indicated that the bleaching in this study was caused by Vibrio infection and the following shift of bacterial community, but not by the dissociation of algal symbionts.

To sum up, this study expands the cognition of the correlation between coral symbiotic Vibrio and coral health. According to the experience of other reported Vibrio pathogens, the outbreak and pathogenicity enhancement of Vibrio may be related to environmental changes (Kimes et al., 2012). The symbiotic changes caused by the outbreak of V. fortis, especially the increased abundance of other pathogenic bacteria, may also cause more serious damage to the coral holobiont. In addition, the reduced abundance of potential probiotics Bacillus under the competition of microbiota might also provide an experimental experience for probiotic strategy (Zhao et al., 2019) or QS regulation (Zhou et al., 2020) on pathogen control or resistance enhancement (Rosado et al., 2019).