To gel or not to gel: differential expression of carrageenan-related genes between the gametophyte and tetasporophyte life cycle stages of the red alga Chondrus crispus

Chondrus crispus is a marine red alga with sulfated galactans, called carrageenans, in its extracellular matrix. Chondrus has a complex haplodiplontic life cycle, alternating between male and female gametophytes (n) and tetrasporophytes (2n). The Chondrus life cycle stages are isomorphic; however, a major phenotypic difference is that carrageenan composition varies significantly between the tetrasporophytes (mainly lambda-carrageenan) and the gametophytes (mainly kappa/iota-carrageenans). The disparity in carrageenan structures, which confer different chemical properties, strongly suggests differential regulation of carrageenan-active genes between the phases of the Chondrus life cycles. We used a combination of taxonomy, biochemistry and molecular biology to characterize the tetrasporophytes and male and female gametophytes from Chondrus individuals isolated from the rocky seashore off the northern coast of France. Transcriptomic analyses reveal differential gene expression of genes encoding several galactose-sulfurylases, carbohydrate-sulfotransferases, glycosyltransferases, and one family 16 glycoside hydrolase. Differential expression of carrageenan-related genes was found primarily between gametophytes and tetrasporophytes, but also between the male and female gametophytes. The differential expression of these multigenic genes provides a rare glimpse into cell wall biosynthesis in algae. Furthermore, it strongly supports that carrageenan metabolism holds an important role in the physiological differentiation between the isomorphic life cycle stages of Chondrus.

. The isomorphic life cycle stages of Chondrus crispus and their dominant carrabiose motifs. The life cycle consists of an alternation between haploid dioecious gametophytes and a diploid tetrasporophyte. After fertilization, the zygote develops within the carposporophyte on the female gametophyte and is mitotically amplified-producing thousands of diploid carpospores that after release will give rise to tetrasporophytes. These carrabiose structures represent the dominant repeating disaccharides found in the Chondrus ECM. Natural carrageenans are hybrid polymers of repeating units, for example Chondrus gametophytes are composed primarily of kappa-and iota-carrageenan motifs (~ 70% and 20%) and the non-cyclized mu-and nu-carrageenan motifs (~ 8% and 2%) 19 www.nature.com/scientificreports/ demonstrate functionally distinct biological signalling properties. The tetrasporophyte susceptibility to infection could also scale up to population-level processes. Indeed, many Chondrus populations are gametophyte-biased. When infection rates were compared with ploidy ratios in natural populations in northwestern France 14 , they were significantly higher in low shore and denser populations that were correspondingly gametophyte-biased. In contrast, on the high shore, where populations are less dense, infections levels were lower and the high shore population was not different from the expected ratio of √ 2:1, due to differential reproduction by females and tetrasporophytes 24,25 .
A pathway for carrageenan biosynthesis was first proposed in 1979 26 and updated in 2015 27 . To date, the only red algal enzymes biochemically characterized in this pathway are the galactose-sulfurylases, which catalyse the formation of 3,6-anhydro-galactose through removal of the C6 sulfate group of galactose ( Fig. 3) 7,28 . These enzymes are unique to red algae and are involved in the last step of carrageenan biosynthesis, controlling the conformation of the polysaccharide chain. Formation of the 3,6-anhydro-bridge from the precursors substrates α-D-galactose-6-sulfate or α-D-galactose-2,6-disulfate to the products α-3,6-anhydro-D-galactose or α-3,6anhydro-D-galactose-2-sulfate, respectively, results in a ring flip from 4 C 1 to 1 C 4 and increases the hydrophobic nature of the monosaccharide moieties. As a tertiary structural consequence, the 3,6-anhydro-bridges promote formation of helices in the carrageenan chain, which then form gel-networks 29 . The in vitro rheological properties of the carrageenans differ depending on the degree of sulfation and presence of 3,6-anhydro-D-galactose. Industry exploits kappa-and iota-carrageenans for their gel forming properties while lambda-carrageenan is used mainly as a thickening agent 30 . Little is known on the in vivo rheological properties of the different carrageenans within the ECM though gametophyte distal tissues are stronger, more extensible and stiffer than tetrasporophyte www.nature.com/scientificreports/ distal tissues 31 . No biomechanical differences were found in the stipe holdfast junctions 31 , suggesting neither gametophytes nor tetrasporophytes have an advantage relative to one another against wave exposure. The molecular composition of the carrageenan metabolites in the ECM is structurally distinct between the life cycle stages, and yet morphologically the Chondrus individuals resemble one another texturally and visually. To the best of our knowledge there are no studies describing differences in carrageenan structure between male and female gametophytes though it would not be unexpected to find molecular differences. In any case, there is strong reason to believe that carrageenan structure plays a role in physiological differentiation during the life cycle of Chondrus. The differences in carrageenan composition between the Chondrus gametophytes and tetrasporophytes [15][16][17][18] suggest that there is differential gene expression of carrageenan-related genes between the life cycles stages. Furthermore, the maintenance of isomorphic haplodiplontic life cycles, such as found in Chondrus, is predicted if the two stages exploit different niches, even if those differences are subtle 32 . Differential gene expression of genes so integral to the structure of the thallus would fit the predictions 32 , but studies explicitly testing this hypothesis are rare 33 . With the available genomic and genetic resources and the accessibility of the different life stages in the field 34 , Chondrus provides an ideal model to address the gene expression in its isomorphic gametophyte and tetrasporophyte stages. Here, we use a combination of taxonomy, biochemistry, molecular biology and transcriptomics to identify select carrageenan-related enzymes that contribute to the physiological differentiation of the ECMs between the life cycle stages and these results are put in the context of the predicted carrageenan biosynthesis pathway 26,27 .

Materials and methods
Sample collection. Three male gametophytes (n), three female gametophytes (n) and three tetrasporophytes (2n) of Chondrus crispus were collected in Roscoff, France at the Pointe de Bloscon (48.726° N-3.969° W) on August 16, 2018 just after low tide ( Table 1). The tissue was cleaned briefly in sterile sea water and pad-  26,27 . Steps that have been experimentally elucidated are highlighted in red 7,28 . Galactose-sulfurylase reactions that have been experimentally elucidated are shown in more detail, that is the conversion of mu-to kappa-, and nu-to iota-carrageenan 7 www.nature.com/scientificreports/ ded dry using paper towels. Life cycle stage was initially assessed through presence of reproductive structures (Fig. 2). Female gametophytes (haploid), male gametophytes (haploid) and tetrasporophytes (diploid) were identified by their reproductive organs: (i) fertilized female gametophytes were identified by the presence of cystocarps, (ii) reproductive male gametophytes were identified by a pinkish to white band of spermatangial sori 3 to 10 mm below the apex 35 and (iii) reproductive tetrasporophytes were identified by the presence of tetrasporangial sori 36 . Carposporophytes, the reproductive structures that remain on the female gametophyte post-fertilization in which the females nurture developing zygotes, were carefully excised from the female gametophytes. Similarly, sori containing tissue was removed from the male gametophyte and tetrasporophyte material. Samples were cleaned with sterile sea water, patted to remove excess liquid and flash frozen in liquid nitrogen on-site for later use.
Resorcinol test. The resorcinol test was performed to provide colourimetric differentiation of tetrasporophyte tissue relative to gametophyte tissue 14,[36][37][38] . A 13.6 mM stock resorcinol solution was prepared by diluting 30 mg of powdered resorcinol in 20 mL of distilled water (stored in the dark). The acetal stock solution was made by adding 8 μL of acetal (1,1-diethoxyethane) to 1992 μL water. The reactive resorcinol-acetal solution was made right before usage, 25 mL of concentrated HCl (37%, commercial) was added to 2.25 mL of the stock resorcinol solution followed by addition of 250 μL of acetal stock solution. Small fragments of the algae, approximately 1 mm × 1 mm, were placed in 1.5 mL Eppendorf tubes then 500 μL of the reactive resorcinol-acetal solution was added. The tubes were incubated for 10 min at 80 °C and then cooled on ice for two minutes followed by qualitative colourimetric evaluation of the staining. Gametophytes result in positive tests and turn the solution a reddish colour, while tetrasporophytes result in a negative test ( Table 2, Supplementary Fig. 1).
RNA extractions. RNA of the nine Chondrus thalli was extracted using a the Qiagen RNeasy Plant minikit and following the manufacturer's protocol. The frozen samples were transferred to 1.5 mL Eppendorf tubes and ground down in liquid nitrogen using a pestle to obtain a fine powder. Lysis buffer (RLT) with 0.04 M DTT (inhibitor of RNases) was added immediately after grinding. The lysates were centrifuged and the supernatants were recovered in new tubes. Ethanol was added to 0.5 V and the samples were loaded over two loads onto RNeasy Mini spin columns which was followed by several wash steps. RNA was eluted with 30 μL RNase free water. Quality and quantity of the samples were determined by measuring the A 260 /A 280 and using a Qubit 2.0 Fluorometer with the Qubit RNA BR assay kit.  43 . Genes were considered to be deferentially expressed if they exhibited at least a twofold difference in expression (FC > = 2) between investigated samples and a false discovery rate (FDR) of < 0.05. The data has been deposited in the SRA database under BioProject ID PRJNA606187. The accession numbers for the raw sequence data are provided in Table 1.

Glycoside hydrolase (GH), glycosyl transferase (GT), galactose-sulfurylase and sulftotransferase (ST) annotations.
Enzymes were first identified by homology with a subset of selected enzymes from each CAZyme (Carbohydrate-active enzyme), sulfurylase or sulfotransferase databank using the local BLAST function with an E value threshold of 1.0E -4 in the program ngKLAST (Korilog). Initial annotations were further verified by BLASTp 44 searches against the UniProtKB/SWISSPROT database, signature scans using InterPro 45 , and HMMER searches against the Pfam database 46 . Whenever possible, each enzyme was assigned to a family.
Phylogeny. Galactose-sulfurylase homologous sequences identified from Chondrus were selected by Blastp at NCBI 47 . The proteins were aligned using MAFFT 48 with the L-INS-I algorithm and the scoring matrix Blo-sum62. The alignment was manually refined using BioEdit 49 . The evolutionary history was inferred by using the Maximum Likelihood method and Whelan And Goldman model 50 . The tree with the highest log likelihood (−5,187.58) is shown. The percentage of trees in which the associated taxa clustered together is shown next to the branches. Initial tree(s) for the heuristic search were obtained automatically by applying Neighbor-Join and BioNJ algorithms to a matrix of pairwise distances estimated using a JTT model, and then selecting the topology with superior log likelihood value. A discrete Gamma distribution was used to model evolutionary rate differences among sites (5 categories (+ G, parameter = 2.1008)). The tree is drawn to scale, with branch lengths measured in the number of substitutions per site. This analysis involved 16 amino acid sequences. There were a total of 263 positions in the final dataset. Evolutionary analyses were conducted using MEGA X 51 .

Results and discussion
Assessment of life cycle stage. The nine Chondrus thalli used in this study were sampled from the rocky intertidal and a morphological determination of ploidy and sex was made in the field based on the presence of reproductive structures (Fig. 2). Gametophytes were also differentiated from the tetrasporophytes by their iridescence, which the tetrasporophytes lack 15 .
To further support the ploidy assessment of the Chondrus individuals we performed the resorcinol test 37,38 . Previous work has shown this test to be reasonably accurate in determining ploidy stage when accompanied by microsatellite genotyping that can distinguish haploid from diploid thalli 14,36 . The colourimetric assay was positive for the male and female gametophytes and negative for the tetrasporophytes supporting the initial morphological assessment of life cycle stage (Table 2, Supplementary Fig. 1).
Microsatellite multilocus genotyping also confirmed ploidy though none of the microsatellites are sex-specific or have sex-specific alleles. All gametophytes exhibited a single allele per locus, whereas the tetrasporophytes had two alleles at five of the six loci used to genotype the thalli (Table 3). At the Port de Bloscon, tetrasporophytes had, on average, 3.9 heterozygous loci out of the same 6 loci genotyped both determined previously 36 and in this study.

Carrageenan biosynthesis. Galactose-sulfurylases. The final step of iota-carrageenan biosynthesis in
Chondrus, namely the conversion of nu-carrageenan to iota-carrageenan (Fig. 3), has been clearly shown in www.nature.com/scientificreports/ Chondrus gametophytes through the biochemical characterization of purified wild type D-galactose-2,6-sulfurylase I and II 7 . There is only one copy of the galactose-2,6-sulfurylase I gene encoded in the Chondrus genome; however, the galactose-sulfurylase II enzymes are one of the rare multigenic families in Chondrus 40 . During the annotation of the differentially expressed genes from Chondrus we identified five new putative galactosesulfurylase II enzymes bringing the total number of Chondrus galactose-sulfurylase II enzymes from 11 40 to 16 (Table 4). An updated phylogenetic analysis on the galactose-sulfurylase II family in Chondrus is shown in an unrooted phylogenetic tree in Fig. 4. The newly identified galactose-sulfurylase II proteins in Chondrus are phylogenetically distant leading us to speculate on differing substrate specificities within the galactose-sulfurylase II family. For example, D-galactose-6-sulfurylase activity, for the enzymatic transformation of mu-carrageenan to kappa-carrageenan (Fig. 3), has been detected in Chondrus extracts 28 though the enzyme(s) have not been identified.
Only one galactose-sulfurylase II gene was significantly upregulated in gametophytes relative to tetrasporophytes (Fig. 5, Table 4, CHC_T00008027001). The same galactose-sulfurylase also showed a significant difference in gene expression between the male and female gametophytes. This enzyme is interesting as it is phylogenetically distant in the galactose-sulfurylase II phylogenetic tree (Fig. 4) suggesting a difference in specificity from the originally identified galactose-sulfurylase II enzymes.
Tetrasporophytes have primarily lambda-carrageenan in their ECM which is depleted in 3,6-anhydrobridges [15][16][17][18] . Unexpectedly, 10 galactose-sulfurylase II genes, encoding enzymes involved in the formation of 3,6-anhydro-bridges 7 , were upregulated in tetrasporophytes relative to the male and female gametophytes. Natural carrageenans are hybrid polymers of different carrabiose repeating units. It is tempting to imagine that the sulfurylase genes expressed during the tetrasporophyte stage are for the formation of highly specialized glycan sequences containing the 3,6-anhydro-D-galactose motif within the lambda carrageenan backbone that forms the mainstay of the carrageenan chains in the tetrasporophytes 17 . These 3,6-anhydro-bridge motifs would induce structural changes in the carrageenan architecture and the specialized carrageenan sequence motifs might also be influential in recognition, signalling or developmental events.
The galactose-sulfurylases are one of red algae's most interesting, yet least understood, family of enzymes and the differential expression of their genes between the red algal life stages underscores the importance of this multigenic family to ECM modification in red algae. More biochemical studies are required to fully understand the fine specificities and unknown catalytic mechanism of this unique enzyme family and to confirm that other members of the family are also involved in 3,6-anhydro-bridge formation.
Glycosyl Transferases (GTs). Unlike land plants, sulfated polysaccharides dominate the extracellular matrices of algae. The other main well of natural sulfated polysaccharides comes from animals; they have a special subset of charged polysaccharides called the glycosaminoglycans or GAGs. Structurally the heterogeneous GAGs are similar to carrageenan, they are long, unbranched, often sulfated, and consist of a repeating disaccharide unit. Many useful and interesting parallels in carrageenan biosynthesis can be extrapolated from the synthesis of animal GAGs 52,53 . Both chondroitin sulfate and heparan sulfate synthesis begin with the stepwise addition of monosaccharides by different glycosyl transferases (GTs) to form a tetrasaccharide linker attached to a core protein. Following linker region synthesis, specific GTs successively add monosaccharides to form the repetitive disaccharide backbone polymer of the GAG. Sulfotransferases (STs) act on the growing polysaccharide chain in a regiospecific manner. Further modifications by other enzymes are also possible.
Several genes, encoding glycosyl transferase enzymes from different CAZy families 54 , were differentially regulated between the life cycle stages of Chondrus. Through manual gene annotation we identified specific GT families we hypothesize to be involved in carrageenan glycosidic bond formation.
Chondrus has four GT7 enzymes whereas the red macroalga Porphyra umbilicalis, which produces the sulfated polysaccharide porphyran in its ECM and whose carbohydrate-active enzymes have been annotated 55 , has only one. The closest non-algal homologues of the GT7s are found in animals 27 and are implicated in GAG biosynthesis, particularly chondroitin sulfate biosynthesis as beta-1,4-N-acetylgalactosaminyltransferases 53 . The relationship to sulfated polysaccharide biosynthesis in animals suggests the red algal GT7 members may also be involved in sulfated carbohydrate biosynthesis and that at least some of the actors involved in sulfated polysaccharide biosynthesis have evolved from the last eukaryotic common ancestor 27,40 . Based on the activities already described in the GT7 family 54 , the GT7 enzymes from Chondrus are predicted to transfer an activated galactose Table 3. Microsatellite results for the Chondrus samples, sizes of the PCR fragments are shown in base pairs.
The three GT47 enzymes from Chondrus are most closely related to plant GT47 members involved in cell wall biosynthesis. Activities described in plants include xyloglucan beta-galactosyltransferase (hemicellulose biosynthesis) 56 , pectin beta-glucuronyltransferase 57 , pectin xylogalacturonan xylosyltransferase 58 and arabinan alpha-L-arabinosyltransferase (pectic arabinan biosynthesis) 59 . GT47 members are also involved in heparan sulfate biosynthesis in animals, adding beta-1,4-glucuronic acid to the growing heparan chain 53 . The relationship to other GT47 enzymes involved in the biosynthesis of negatively charged (pectin and heparan sulfate) and sulfated (heparan sulfate) extracellular glycans leads to the prediction that these enzymes are implicated in carrageenan chain elongation in Chondrus. It is difficult to assign a more specific annotation based on the diverse Table 4. Annotated carrageenan-biosynthesis genes. Averaged TPMs are shown for the Chondrus female and male gametophytes and the tetrasporophytes. The differential gene expression is shown for the pairwise comparisons between the life cycle stages. Significant differences are marked with an asterisk. F is female gametophyte, M is male gametophyte, and T is tetrasporophyte.

Gene Annotation
Gene expression level (TPM) www.nature.com/scientificreports/ activities already described in the GT47 family. There is one GT47 member from Chondrus that is significantly upregulated ( Table 4, Fig. 5) in tetrasporophytes relative to gametophytes (CHC_T00009549001). The GT47 gene CHC_T00009415001 shows higher expression levels in the gametophytes which is significant in the female gametophytes relative to the tetrasporophytes (Table 4, Fig. 5).
There are six Chondrus GT14 enzymes and four Porphyra GT14 enzymes that find their closest non-algal homologues in plant GT14 enzymes. Three Arabidopsis thaliana enzymes have been characterized from plants and all are implicated in type II arabinogalactan biosynthesis in the cell wall, acting as β-1,6-glucuronosyltransfer ases 60,61 , transferring a negatively charged glucuronic acid molecule to galactan oligosaccharides. Metazoan GT14 enzymes have demonstrated β-1,6-N-acetylglucosaminyltransferase activity, forming crucial side chain branches in core 2 mucin O-glycans 62 and the blood group I-antigen during embryonic development 63 , as well as peptide O-β-xylosyltransferase activity, essential as the first step in the biosynthesis of chondroitin, dermatan and heparan sulfate 64 . Involvement of the GT14 family in negatively charged and sulfated glycan biosynthesis suggests that the Chondrus enzymes are implicated in carrageenan biosynthesis and that the Porphyra enzymes are implicated in porphyran biosynthesis. It is difficult to predict a specific activity though the Chondrus GT14 enzymes may be involved in chain initiation or elongation in carrageenan biosynthesis. There are three GT14 members that www.nature.com/scientificreports/ have higher gene expression in tetrasporophytes relative to gametophytes (Table 4, Fig. 5). Conversely, one GT14 is upregulated in the gametophytes which is significant for the female relative to the tetrasporophytes (Table 4, Fig. 5). In both plants and animals, the GT14 enzymes have demonstrated important roles in development and this might hold true in red algae as well.
Carbohydrate-Sulfotransferases. Carboydrate sulfotransfereases (STs) act by adding sulfonyl groups from 3′phosphoadenosine-5′phosphosulfate (PAPS) to a glycoside receptor 65 . Chondrus has seven predicted carbohydrate-STs with their non-algal ST homologues found in animals and active in GAG sulfations. Comparatively, Porphyra has only one carbohydrate-ST, likely active as an L-galactose-6-O-sulfotransferase in the biosynthesis of porphyran 55 . Brown algal carbohydrate-STs also share an evolutionary relationship with animal STs involved in GAG biosynthesis 66 . Land plants, which don't grow in a saline environment, aren't known to have sulfated polysaccharides and lack the STs common to animals and algae. Sea plants, such as the seagrass Zostera marina 67 , have regained capability to sulfate their polysaccharides through unknown mechanisms. Overall, the evolutionary relationship between animal carbohydrate-STs and algal STs lends support to the ancestral nature of sulfated polysaccharide biosynthesis in eukaryotes. Carrageenan is the only known sulfated carbohydrate in Chondrus, thus it remains the prime substrate candidate for the carbohydrate-ST family of enzymes 65 . Carbohydrate-STs tailor the physico-chemical and mechanical properties of the algal ECM providing both elasticity and strength which intuitively would help protect against the strong ocean currents 68 . In animals, diverse regiospecific sulfation patterns on GAGs are both structural and a source of extracellular biological information to cells, influencing recognition events, signalling pathways and developmental processes 65,69,70 . In analogy to the animal GAGs 69,70 , these specialized carrageenan sulfations sequence motifs may also be important for recognition, signalling or development events in algae. Unlike animals, sulfatases have not yet conclusively been identified or characterized in red algae. It is unknown how red algae cope with ECM remodeling in the absence of known sulfatases, though the red algal microbiome has a role in the recycling of sulfur as it produces sulfatases specific for carrageenan [71][72][73][74] .
Altogether, five carbohydrate-ST enzymes were differentially regulated between the Chondrus life cycle stages ( Table 4, Fig. 5). Four of the carbohydrate-ST genes were differentially expressed between the gametophytes and the tetrasporophytes. This suggests major differences in sulfation patterns between the gametophyte and tetrasporophyte life stages, which is supported in the literature [15][16][17][18] .
Glycoside hydrolases. Glycoside hydrolases are enzymes that hydrolyze the glycosidic bond through the addition of a water molecule and in some specialized instances they may act as transglycosidases, forming a glycosidic bond. Chondrus has three genes encoding family 16 glycoside hydrolases (GH16). A phylogeny on the GH16 family has been previously undertaken and the three GH16 members from Chondrus (CcGH16-1, CcGH16-2 and CcGH16-3) are found in the same clade as bacterial agarases, porphyranases and three red algal enzymes from Porphyra 55 . Red algae likely obtained these genes through a horizontal gene transfer event between marine bacteria and red algae 55 . Since agar and porphyran are not present in the ECM of Chondrus, the function of the www.nature.com/scientificreports/ Chondrus GH16 enzymes may be in the remodeling of its own sulfated ECM polysaccharide, carrageenan. The gene expression for one family 16 glycoside hydrolase was upregulated both in male gametophytes and tetrasporophytes relative to the female gametophytes (Table 4, Fig. 5). This interesting result suggests molecular differences in carrageenan structure between male and female gametophytes.

Conclusion
Carrageenan biosynthesis between the life cycle phases implicates the differential regulation of several rare multigenic gene families in Chondrus. Carrageenan can, at times, make up over 50% of the dry weight of Chondrus 18 , highlighting the importance of the carrageenan macromolecule to the success of this red alga. Here, we demonstrate that carrageenan biosynthesis in these multigenic families is at least partially regulated through modulation of gene transcription between the life cycles in Chondrus, indicating a level of genetic control. This genetic control is likely at least partially responsible for the molecular differences in carrageenan structure between the tetrasporophyte and gametophyte isomorphic life cycle stages. The foremost differences in carrageenan-related gene expression between life cycle stages is seen between the gametophytes and the tetrasporophytes. Thus, the differential regulation of the carrageenan-utilization genes between life stages may be important for the biosynthesis of specialized glycan motifs within the polymer. Only two genes, CcGH16-3 and a galactose-sulfurylase II (CHC_T00008027001), showed differential gene expression between the male and female gametophytes. Male and female gametophytes have been described as having similar carrageenan structures; however, these differential gene expression results suggest some differences in architecture. This also supports data from infection experiments with the pathogen Ulvella operculata in which male gametophytes were found to be slightly more infected than female gametophytes, though never to the level of tetrasporophytes 23 . Male gametophytes shed their apices following spermatial release 35 and generally look more tattered than the female gametophytes (SA Krueger-Hadfield, personal observation). No studies have explored in detail the male gametophytes in natural populations of Chondrus. Differences in carrageenan structure may manifest at the population level though more work is necessary to link these data to field-patterns in ploidy and sex ratios. For example, if there are differences between male gametophyte, female gametophyte, and tetrasporophtye infection rates linked to carrageenan content, as has been suggested 6,23 , then there may be corresponding differences in abundances of thalli in the field due in part to infection-induced dislodgement. Not only do our data support the hypothesis of niche partitioning between Chondrus life cycle stages, by providing evidence of differential gene expression governing the physiological state of gametophytes and tetrasporophytes 32 , they pose excellent topics for further investigation. Future studies, exploring niche differentiation and underlying genetic components, could shed light on the maintenance of haplodiplontic life cycles and contribute to understanding the concept of the niche that is relevant for the organism in question.
Altogether, these data strongly support that macromolecular structure of carrageenan in the ECM of Chondrus correlates to the physiological differentiation of the alga throughout the isomorphic life stages.