Biocalcification in porcelaneous foraminifera
eLife assessment
This manuscript provides important information on the calcification process, especially the properties and formation of freshly formed tests (the foraminiferan shells), in the miliolid foraminiferan species Pseudolachlanella eburnea. The evidence from the high-quality SEM images is convincing although the fluorescence images only provide indirect support for the calcification process.
https://doi.org/10.7554/eLife.91568.3.sa0Important: Findings that have theoretical or practical implications beyond a single subfield
- Landmark
- Fundamental
- Important
- Valuable
- Useful
Convincing: Appropriate and validated methodology in line with current state-of-the-art
- Exceptional
- Compelling
- Convincing
- Solid
- Incomplete
- Inadequate
During the peer-review process the editor and reviewers write an eLife Assessment that summarises the significance of the findings reported in the article (on a scale ranging from landmark to useful) and the strength of the evidence (on a scale ranging from exceptional to inadequate). Learn more about eLife Assessments
Abstract
Living organisms control the formation of mineral skeletons and other structures through biomineralization. Major phylogenetic groups usually consistently follow a single biomineralization pathway. Foraminifera, which are very efficient marine calcifiers, making a substantial contribution to global carbonate production and global carbon sequestration, are regarded as an exception. This phylum has been commonly thought to follow two contrasting models of either in situ ‘mineralization of extracellular matrix’ attributed to hyaline rotaliid shells, or ‘mineralization within intracellular vesicles’ attributed to porcelaneous miliolid shells. Our previous results on rotaliids along with those on miliolids in this paper question such a wide divergence of biomineralization pathways within the same phylum of Foraminifera. We have found under a high-resolution scanning electron microscopy (SEM) that precipitation of high-Mg calcitic mesocrystals in porcelaneous shells takes place in situ and form a dense, chaotic meshwork of needle-like crystallites. We have not observed calcified needles that already precipitated in the transported vesicles, what challenges the previous model of miliolid mineralization. Hence, Foraminifera probably utilize less divergent calcification pathways, following the recently discovered biomineralization principles. Mesocrystalline chamber walls in both models are therefore most likely created by intravesicular accumulation of pre-formed liquid amorphous mineral phase deposited and crystallized within the extracellular organic matrix enclosed in a biologically controlled privileged space by active pseudopodial structures. Both calcification pathways evolved independently in the Paleozoic and are well conserved in two clades that represent different chamber formation modes.
Introduction
Over the past 500 million years, living organisms evolved different skeleton crystallization pathways. Very popular in nature is the mineralization of the extracellular matrix, e.g., in crustacean cuticles, mollusk shells, vertebrate bones, and teeth composed of dentin and enamel (Weiner and Addadi, 2011; Kahil et al., 2021; Ujiié et al., 2023). Radial foraminifera represented by rotaliids have been traditionally interpreted to make use of this crystallization mode (Weiner and Addadi, 2011). The other two pathways are intravesicular and are characterized by either production of amorphous unstable phase within a large vesicle, such as a syncytium, well documented for sea urchin larvae (Beniash et al., 1997) or crystallization of calcite elements within smaller vesicles located in the intracellular space, as seen in fish that form guanine crystals and coccolithophores to produce coccoliths (Weiner and Addadi, 2011; Kahil et al., 2021). This model has also been attributed to the formation of porcelaneous shells by miliolid foraminifera (Weiner and Addadi, 2011) based on the model proposed by Berthold, 1976, and followed by .
As such, mineralization of shells in Foraminifera is believed to follow two highly contrasting pathways. The current theory states that Miliolida, characterized by imperforate, opaque milky-white shell walls (porcelaneous) (Angell, 1980; de Nooijer et al., 2009), produce fibrillar crystallites composed of Mg-rich calcite within tiny vesicles enclosed by cytoplasm. Miliolid shells are made of randomly distributed calcite needles that form a dense meshwork of chaotic crystallites that cause light reflection, resulting in opaque (porcelaneous) milky walls (Hohenegger, 2009). Calcite needles are thought to be precipitated completely within these vesicles and then transported to the site of chamber formation to be released via exocytosis (Berthold, 1976; Angell, 1980; de Nooijer et al., 2009; de Nooijer et al., 2008). The pre-formed needles or needle stacks are believed to be continuously embedded in an organic matrix (OM) in the shape of the new chamber until the wall is completed. Although this model is commonly accepted, it has never been sufficiently documented in vivo, and it does not resolve several conflicting issues. First of all, the question is how pre-formed bundles of parallel calcitic needles are transformed into randomly oriented needles within the shell wall. It is difficult to explain, if there is no recrystallization process within the wall structure after discharging the calcite crystallites. This problem was already emphasized by Hemleben et al., 1987. Second, why the newly constructed wall is still translucent after deposition of random crystals. We would expect a thin milky opaque layer of the new wall under normal transmitted light, as well as polarized crystals of calcite under crossed nicols. Angell, 1980, on his plate 2 presenting porcelaneous chamber formation in miliolid Spiroloculina hyalina Schulze clearly documented the polarization front being shifted circa a half of the length of the new chamber behind the leading edge of the forming chamber. This shift represented more than an hour. Therefore, polarization was missing in the early and middle stage of chamber formation. It means that Angell, 1980, time lapse micrographs of the chamber formation were in conflict with the imaging under TEM. It seems that Angell, 1980, was aware of that problem and stressed that calcification had to be “intense enough to show under crossed nicols lags behind the leading edge of the forming chamber” (p. 93, pl. 2 figure 12/caption). In fact, all experiments that show the ‘crystal vacuoles’ (sensu Angell, 1980) documented under TEM (Berthold, 1976; Angell, 1980) required fixation of the samples, which was prone to post-fixation artifacts of unwanted calcite precipitation.
Our goal is to test whether the miliolid shell is produced by ‘agglutination’ of premade needle-like calcitic crystallites, and in consequence, whether this large group of calcareous Foraminifera follow crystallization within smaller vesicles located in the intracellular space. Therefore, we re-examined the mineralization process in Miliolida based on experiments on a living species, Pseudolachlanella eburnea (d’Orbigny) (Figure 1). This taxon was selected to facilitate replicated observations of chamber growth under controlled culture conditions. We included observations of in vivo biomineralization using multiphoton and confocal laser scanning microscopy (CLSM) followed by analyses of fixed specimens at different stages of chamber formation by high-resolution field emission scanning electron microscopy (FE-SEM) coupled with energy-dispersive X-ray spectrometry (EDS). Our new FE-SEM data challenge the current understanding of the biomineralization of miliolid foraminifera and such a significant divergence of biomineralization pathways within the Foraminifera.
Results
All replicated in vivo experiments on P. eburnea facilitated by CLSM imaging with the application of membrane-impermeable Calcein and FM1-43 membrane dyes (performed in separate experiments) showed intravesicular fluorescence signals from groups of moving vesicles (1–5 µm in size) inside the cytosol (Figure 2A and B, Figure 2—video 1 and Figure 2—video 2). The fluorescent vesicles inside the cytosol contained seawater, as documented by fluorescence of membrane-impermeable Calcein. These vesicles were taken up by endocytosis indicated by FM1-43 staining. This dye stains the cell membranes and indicates all endocytic vesicles by fluorescence, whereas the other intracellular vesicles remain unstained (Amaral et al., 2011). Both dyes demonstrate the uptake of seawater via the endocytosis of vesicles that are approximately 1–4 µm in diameter and move through the entire cell.
Additional LysoGlow84 staining revealed numerous acidic vesicles in the cytosol (Figure 2C, Figure 2—video 3 and Figure 2—video 4). Acidic vesicles were accompanied by other vesicles (approximately 1–2 µm in size) that show autofluorescence upon multiphoton excitation at 405 nm (emission 420–480 nm), shown in red in Figure 2C. This wavelength partly permeates the shell to excite autofluorescence interpreted as associated with ACCs (see Dubicka et al., 2023). The autofluorescence of the shell itself is also present (Figure 2D), however, it is not clearly visible because the fluorescence of ACCs is much stronger. The intensity of the laser light is reduced because the multiphoton light has to pass through a thick three-dimensional carbonate wall of the foraminiferal shell. Further experimental studies are needed to confirm the ACC source of this autofluorescence and thus definitively eliminate potential organic sources of AF emissions.
In addition, typical chlorophyll autofluorescence (excitation at 405 or 633 nm, emission 650–700 nm, Figure 2C, Figure 2—video 3 and Figure 2—video 4 highlighted in green) was detected, which indicated the presence of chloroplasts in microalgae cells. These algal cells have been found to move within the cytosol of the observed specimens, in proximity of acidic vesicles and vesicles characterized by autofluorescence upon UV light (exc. 405 nm). These algal cells may represent facultative endosymbionts, as they were observed only during the chamber mineralization process in specimens with carbonate-bearing vesicles likely detected by in vivo CLSM experiments. They were documented just below the OM of the newly formed chamber, as seen in the FE-SEM observations as well as just below the OM of the newly created chamber as seen in the FE-SEM observations (Figure 3—figure supplement 1G and H). Specimens of P. eburnea, which displayed vesicles showing autofluorescence under UV light inside the cytosol, were fixed using Method B (see Materials and methods) coated with a few nanometers of carbon and analyzed by SEM-EDS. The main elements detected in the area of the fixed cytoplasm (Figure 3—figure supplement 4) were C, O, Na, Mg, P, S, Cl, K, and Ca (of particular interest were the high contents of Mg and Ca), whereas the main elements detected within the area of the new chamber in the form of a gel-like matter filled with dispersed nanograins were C, O, Na, Mg, S, Cl, and Ca (Figure 3—figure supplement 4). The shell content was strongly enriched with Ca relative to the cytoplasm, which showed a much higher Mg/Ca ratio.
FE-SEM observations of the fully mineralized test walls displayed the porcelaneous structures (see Parker, 2017; Dubicka et al., 2018), which are made of three mineralized zones, i.e., (1) extrados that represents an outer mineralized surface (approximately 200–300 nm in thickness; Figure 3—figure supplements 1C and 2C); (2) porcelain that denotes the main body of the wall constructed from randomly oriented needle-shaped crystals (up to 1–2 μm in length and approximately 0.2 μm in width). No gel-like matter was observed between the needles of the porcelain structures that appeared in the early stages of wall formation (Figure 3E, E1; Figure 3—figure supplements 2C and 3A); and (3) intrados that represents an inner mineralized surface (approximately 200–300 nm in thickness) made of needle-shaped crystallites (Figure 3E, E1 and Figure 3—figure supplement 1A).
Growing chambers, captured at the various successive stages of chamber formation in different specimens, have revealed the following morphological features: (1) a solitary, thin organic sheath (approximately 200–300 nm thick) that represents the most distal part of the new chamber and is anchored to the older, underlying solid calcified chamber (Figure 4A); (2) a solitary, outer organic sheath (OOS) filled with spread calcifying nanograins (Figure 4B; Figure 3—figure supplement 2); (3) a gel-like matter (4–5 µm in thickness) with a granular texture, bounded on two sides by intrados and extrados, and containing relatively widely spaced, randomly dispersed carbonate nanograins (Figure 3A, B; Figure 4C; Figure 3—figure supplement 1A–D); (4) the test inside made of chaotic meshwork of carbonate nanograins partly transformed to short needles with a small amount of gel-like OM in-between (Figures 3C, D, 4D); (5) the test inside composed of needle-shaped crystals with planar faces and no apparent remaining gel-like matter (Figures 3E, E1, 4E). Carbonate nanograins at the shell construction site were well documented in our SEM-EDS studies (Figure 3—figure supplement 4). Both fixation methods (see Materials and methods) yielded highly consistent results.
Discussion
Porcelaneous shell formation
Comparative analysis of the nanostructures of the newly built chambers combined with the elemental composition obtained from SEM-EDS, as well as the data from CLSM, allowed us to identify important steps in the accretive formation of P. eburnea shells. The formation of a new chamber begins with the construction of a thin OOS that pre-shapes the new chamber (Figures 4A and 5). The OOS is made by pseudopodial structures supported by the cytoskeleton immediately after the extrusion of a small mass of cytoplasm from the aperture (Figure 1E and F). Once the OOS is constructed, the first calcium carbonate accumulation takes place inside in the form of carbonate nanograins (Figures 4B and 5, Figure 3—figure supplement 2A and B), creating the extrados. The extrados stabilizes the final chamber morphology relatively quickly. Subsequently, the wall gradually thickens through the primary accumulation of hydrated and amorphous Mg-rich CaCO3 (Figures 4B and 5). We suppose that the carbonate content is successively deposited by exocytosis of Mg-ACC-rich vesicles that most likely represent the vesicles converted from seawater stained with Calcein (Figure 5). The characteristic autofluorescence inside foraminiferal cell excited at 405 nm (Figure 2; Figure 2—video 3 and Figure 2—video 4) most likely indicates the carbonate content of the vesicles, which are considered to be Mg-ACCs (see Dubicka et al., 2023). Mg-ACC is an unstable, amorphous and hydrated form of CaCO3 with a significantly high concentration of Mg (Raz et al., 2000; Weiner et al., 2003; Bentov and Erez, 2006; Kahil et al., 2021) and is commonly regarded as a resource for most biocalcification processes. ACCs have been found in many calcifying marine organisms, such as echinoderms, mollusks, coccolithophorid algae, cyanobacteria, crustaceans, and rotaliid foraminifera, where they are typically interpreted as pre-material phases for the production of calcite skeletons (Hasse et al., 2000; Weiss et al., 2002; Sviben et al., 2016; Dubicka et al., 2018; Kahil et al., 2021). Research suggests that a high-Mg content not only makes ACC unstable but also facilitates the transport of ACC to the crystallization site, where it is initially transformed into carbonate nanograins (Cölfen and Qi, 2001; Addadi et al., 2003; Raz et al., 2003; Dubicka et al., 2023). The existence of intracellular, vesicular intermediate amorphous phase (Mg-ACC pools), which supplies successive doses of carbonate material to shell production, might be supported not only by autofluorescence (excitation at 405 nm; Figure 2; Figure 2—video 3 and Figure 2—video 4; see Dubicka et al., 2023) but also by a high content of Ca and Mg analyzed in the cytoplasmic area by SEM-EDS analysis (Figure 3—figure supplement 4). In the future, more precise higher resolution elemental measurements are needed for better documentation of miliolid ACC-bearing vesicles. However, the small size of carbonate-bearing vesicles (approximately 1–2 µm) may make this difficult.
Mg2+ and Ca2+ ions for intravesicular production of Mg-ACCs are obtained from seawater and taken up by endocytosis, as independently indicated by membrane-impermeable Calcein, as well as by the FM1-43 probe selectively labeling membranes of endocytic vesicles (Figure 2A and B, Figure 2—video 1 and Figure 2—video 2). We hypothesize that vesicles are carried along cytoskeletal structures to the OM, as observed in rotaliid foraminifera (Dubicka et al., 2023), where they dock and release their contents (Figure 4). The nanograins then precipitate within the gelatinous matter that consists of amorphous carbonates and OM released from the vesicles (Figure 3A–C; Figure 4C; Figure 5). Nanograins immersed in the gel-like matter gradually grow into needle-shaped elements, precipitating in situ within the final wall structure (Figure 3C, D; Figure 4D). The gel-like matter appears to be involved in needle formation; however, the OM seems to disappear (Figures 3E and 4E) when the needle-shaped crystals are created. We suspect that the gel-like matter consists of pre-formed liquid amorphous mineral phase (Mg-ACC) within the extracellular OM that is suggested by the EDS spectra of the early stage of the wall calcification (Figure 3—figure supplement 4: A3 area). The calcification of extrados and intrados occurs before the interior of the wall crystallizes, providing stability to the new chamber at both edges of the wall (Figure 4D).
The protruding cytoplasm appears to immediately form a chamber wall by secreting OM and crystals from the vesicles (Angell, 1980). As calcite secretion continues along the leading edge, the newly formed segment remains covered by a thin, moving sheet of cytoplasm that is called by Angell, 1980, the ‘active sheet’. This thin active sheet of cytoplasm may represent a lamellipodium that is a pseudopodial structure known to be involved in the biomineralization of Rotaliida (Tyszka et al., 2019). It is also likely that reticulopodial structures (that do not coat the whole calcification site) are responsible for the distribution and shape of the internal surface of the chamber wall. That occurs by successive accumulation of ACC and OM as identified on TEM images by Angell, 1980. His results suggest that crystallization of calcite needles is ‘limited to a confined space controlled by active cytoplasmic structures’ that are strictly separated by the membranes from the cytosol.
Formation of shell crystallites: a paradigm shift
Miliolids were thought to share a similar, intracellular, crystallization pathway as the coccolith formation in coccolithophorids (Weiner and Addadi, 2011) that evolved in the Triassic, i.e., ca. 210 Myr ago (Gardin et al., 2012). Coccoliths are produced within intracellular Golgi-derived vesicles and then exported to the surface of the extracellular coccosphere (Borman et al., 1986). Miliolids, with their unique fibrillar calcitic microstructures, evolved much earlier, i.e., ca. 300 Myr ago in the late Paleozoic (Figure 3—figure supplement 5). Until now, it was generally considered that calcite crystals in miliolids also precipitate within vesicles immersed in the cytoplasm and are then transported to the location of the wall construction, where they are released by exocytosis (Berthold, 1976; Angell, 1980; de Nooijer et al., 2009; Weiner and Addadi, 2011). Our FE-SEM study of P. eburnea shows the lack of premade needle-like crystallites of calcite at the early stages (I–IV) of the wall formation. In contrast, we can clearly infer the in situ calcification front with a progressive sequence of crystal growth behind the leading edge of the forming chamber (Figures 4 and 5). Therefore, this miliolid species apparently does not produce shells by ‘agglutination’ of premade needle-like crystallites of calcite, in contrast to the traditional miliolid calcification model (Berthold, 1976; Angell, 1980).
In the light of these results, another argument emerges that further confirms in situ calcification of miliolid chambers. It explains the extended transparency of unmineralized walls observed under the light stereomicroscope. The chamber wall under formation tends to gradually change its appearance during calcification from completely transparent to milky and opaque (Figure 1E and F).
Our results on biomineralization of this miliolid species do not confirm the formation of individual skeletal crystallites within intracellular vesicles. However, in turn, our results do support existence of endocytotic vacuolization of seawater in miliolids that was first suggested by . We further support Angell, 1980, interpretation that the calcite crystals are dispersed in the gel-like OM (see Figure 3A, B; Figure 4C, D; Figure 5). This gel-like fluidal OM likely includes a rich Mg-ACC component as the substrate for in situ calcification (Figures 3—5). Interestingly, the previous studies by Angell, 1980, did not support crystal formation within vacuoles either.
Precipitation of calcite nanograins, which then merge and transform into crystallites, probably occurs within the organic matter after the release of Mg2+ from Mg-ACC. The organic matter provides an appropriate physiochemical microenvironment for initiating and maintaining the crystallization process by manipulating many essential factors, including pH, and kinetics of the system (Kahil et al., 2021). According to Tyszka et al., 2021, the OM involved in the biomineralization of foraminiferal miliolid shells may contain collagen-like networks.
Our in vivo CLSM observations show a miliolid cytoplasm containing intracellular carbonate-bearing vesicles. Such vesicles have been well documented by Angell, 1980, who stressed their crucial role in the biomineralization process. However, rather than transporting pre-formed solid needles, the vesicles likely carry liquid or quasi-liquid calcification substrates. This liquid carbonate phase was apparently maintained by a relatively high concentration of Mg (Figure 3—figure supplement 4), which was much higher than that in the shell, as detected by the SEM-EDS analyses.
Recently, an independent study was performed on another miliolid species – Sorites orbiculus (Nagai et al., 2023). The researchers reported highly complementary results that indicate the lack of crystal-like structures within the intracellular vesicles. Their results suggested that calcification of this miliolid species did not follow Hemleben et al., 1987 model because intracellular vesicles did not produce needle-like crystals to construct the shell wall. They also stated that their observations ‘may reveal a novel and unknown mode of biomineralization in foraminifera’.
Because, miliolid wall texture originated together with the appearance of miliolid foraminifera as it has also been recorded within Paleozoic taxa (Figure 3—figure supplement 5), thus the calcification mode of miliolids apparently evolved in the late Paleozoic (≥350 Mya) and is well conserved in this clade till today. It should be emphasized that our recent understanding of all calcification pathways in Foraminifera implies their independent evolution within main phylogenetic groups, besides miliolids and rotaliids, also including spirillinids, nodosariids, and robertinids (Pawlowski et al., 2013; Mikhalevich, 2013; Dubicka et al., 2018; Dubicka, 2019; Sierra et al., 2022; de Nooijer et al., 2023). In fact, most of these biomineralization evolutionary transitions from agglutination to calcification originated in the mid- and late Paleozoic.
Mg-ACC has also recently been documented in rotaliid foraminifera (Mor Khalifa et al., 2018; Dubicka et al., 2023). Therefore, the biocalcification processes in Rotaliida and Miliolida, which belong to the two main foraminiferal classes Globothalamea and Tubothalamea, respectively (Pawlowski et al., 2013), are more alike than previously thought (Weiner and Addadi, 2011). Their mesocrystalline chamber walls are created by accumulating and assembling nanoparticles of pre-formed liquid amorphous mineral phase. Their calcification occurs within the extracellular OM enclosed in a biologically controlled privileged space by active pseudopodial structures. However, we are aware that this process must also vary to some extent as the chemical composition of the calcite, as well as primary crystallite geometries differ between the groups. Seawater provides the relevant Ca and Mg ions for calcification, which are taken up in both groups by endocytosis. In Amphistegina (Rotaliida), this process is performed by shell pores (Dubicka et al., 2023), as well as aperture; in non-porous Miliolida, it is done by granuloreticulopodia emanating from the aperture (Figure 2, Figure 2—video 2). In both the rotaliid Amphistegina and the miliolid P. eburnea carbonate-bearing vesicles are surrounded by moving acidic vesicles (Figure 2, Figure 2—video 3 and Figure 2—video 4), which likely facilitate pH regulation at the mineralization front (see Toyofuku et al., 2017; Chang et al., 2023). It is very likely that pH is controlled by active outward proton pumping by a V-type H+ ATPase or proton outflux driven by pH that is responsible for the proton flux and related calcification (Toyofuku et al., 2017; see also Matt et al., 2022). We suspect much higher pH values within vesicles transporting Mg-ACC to the site of calcification. Such alkaline vesicles were detected by the HPTS fluorescent labeling and reported by several previous studies (de Nooijer et al., 2008; de Nooijer et al., 2009).
Our findings are in line with recent work in biomineralization, supporting that ‘biominerals grow by the accretion of amorphous particles, which are later transformed into the corresponding mineral phase’ (Macías-Sánchez et al., 2011; see also Meldrum and Cölfen, 2008). Miliolid needles, assembled with calcite nanoparticles, are unique examples of biogenic mesocrystals (see Cölfen and Antonietti, 2005), as they form distinct geometric shapes limited by planar crystalline faces. Mesocrystals are constructed from highly ordered individual nanoparticles (Cölfen and Mann, 2003; Sturm (née Rosseeva) and Cölfen, 2016; Sturm (née Rosseeva) and Cölfen, 2017) that form hierarchically structured solid materials in the crystallographic register and are rather devoid of outer planar surfaces. These result from the aggregation, self-assembly, and mesoscopic transformation of amorphous precursor nanoparticles. Mesocrystals are common biogenic components in the skeletons of marine organisms, such as corals, echinoderms, bivalves, sea urchins, and rotaliid foraminifera (e.g. Macías-Sánchez et al., 2011; Benzerara et al., 2011; Seto et al., 2012; Evans, 2019; Dubicka et al., 2023).
Our biomineralization model further explains the random orientation pattern of the calcite needles within the shell wall. The miliolid intertwined calcitic structure cannot be explained by the models proposed by Berthold, 1976, and followed by , i.e., by the successive deposition of vesicles with ready bundles of solid calcitic fibers (needles) without additional recrystallization processes. In our proposed in situ calcification model, calcite crystallites have sufficient space to grow within the flexible gelatinous OM. In addition, our model explains the need for a light and dark phase for the algae that are present inside P. eburnea during the biomineralization processes, as these algae possibly play an important role. Small miliolid coiling foraminifera has been regarded as a non-symbiotic taxon because their shells are not transparent, however, this is not true for red and infrared light. Fully developed miliolid shells are made of randomly distributed needles that cause light reflection, resulting in opaque (porcelaneous) walls that possibly protect the foraminifera from UV irradiation and allow them to live in extremely illuminated shallow seas (Hohenegger, 2009). These walls are permeable to red and infrared light, as we observed using multiphoton laser. Red light is commonly believed to be the most efficient waveband for photosynthesis, however green light may achieve higher quantum yield of CO2 assimilation and net CO2 assimilation rate (Liu and van Iersel, 2021). P. eburnea may acquire its facultative symbionts only for the duration of the biomineralization process. The late stage of needle formation in the shell production process ensures that the wall remains transparent by the time the needles are completed. Similar patterns of the gradual change from transparent to opaque whitish walls were also observed in larger symbiotic miliolids by Marshalek, 1969, Wetmore, 1999, and Tremblin et al., 2021. The latter authors (Tremblin et al., 2021) documented chamber formation of miliolid Vertebralina striata with cytoplasm enveloped by a transparent sheath decorated with striate already present in the transparent wall before calcification. They also interpret white areas on the sheath, indicating incipient concentrations of minute calcite crystallites that represent the mineralized wall. The biomineralization process is likely aided by their dark respiratory activity (see Hallock, 1999), as they could supply calcification substrates such as HCO3- through respiration or by increasing pH at the calcification site during the light phase. Similarly, representatives of miliolid large benthic foraminifera (Archaiasidae, Soritidae, and Peneroplidae) host endosymbiotic algae (Lee, 2006; Prazeres and Renema, 2019). Therefore, they have developed additional morphological and textural features such as pits, grooves/striate, or windows, which enable light penetration into the places where symbionts are positioned (see Hohenegger, 2009; Parker, 2017).
Materials and methods
Living foraminifera, collected from the coral reef aquarium in the Burgers’ Zoo (Arnhem, Netherlands), were cultured in a 10 L aquarium containing seawater with a salinity of 32 psu, pH of 8.2, and a temperature of 24°C. Specimens of P. eburnea (d’Orbigny) were placed in 4 mL Petri dishes 1 day prior to CLSM studies, incubated without food for 18–24 hr, and then individuals that underwent chamber formation were observed under a Zeiss Stemi SV8 stereomikroscope for selection of individuals.
These selected individuals were studied in vivo using a Leica SP5 Confocal Laser Scanning Microscope equipped with an argon, helium-neon, neon, diode, and multiphoton Mai Tai laser (Spectra-Physics) at the Alfred-Wegener-Institut, Bremerhaven, Germany. In vivo experiments were performed by labeling samples with different fluorescent dyes (Table 1) just before imaging using pH-sensitive LysoGlow84 (50 µM exc. MP 720 nm exc./em. 380–415 nm and 450–470 nm, Marnas Biochemicals Bremerhaven, incubation time: 2 hr), FM1-43 membrane stain (1 µM, exc. 488 nm em. 580–620 nm, Invitrogen, incubation time: 24 hr), and membrane-impermeable Calcein (0.7 mg/10 mL, exc. 488 nm, em. 510–555 nm, incubation time: 24 hr). The foraminifera were removed from the Petri dish with clean water using a pipette. In addition, the autofluorescence of specific foraminiferal structures at the chosen excitation/emission wavelength was detected. All experiments were replicated with at least several individuals of the same species. All fluorescence probe experiments were performed with appropriate controls.
Additional foraminifera individuals that had been studied by CLSM were fixed for further analysis. The fixation process followed two different methods: (1) 60 individuals were transferred to 3% glutaraldehyde for 5 s and then dehydrated stepwise for a few seconds with an ethanol/distilled water mixture with increasing concentrations (30%, 50%, 70%, and 99%). (2) The seawater was removed from 50 individuals by pipetting and applying a small piece of Kimtech lab wipe (without any rinsing), followed by quick drying in warm air (30–35°C). This method stops the dissolution of the amorphous mineral phase because there is no contact with other liquids. Fixed foraminifers of both procedures were gently broken using a fine needle to coat the cross-sectional surfaces and tested inside with a few nanometers of either gold or carbon. Foraminifera were then studied using a Zeiss Sigma variable-pressure FE-SEM equipped with EDS at the Faculty of Geology, University of Warsaw.
Data availability
All data generated or analysed during this study are included in the manuscript and supporting files.
References
-
Test morphogenesis (chamber formation) in the foraminifer Spiroloculina hyalina SchulzeThe Journal of Foraminiferal Research 10:89–101.https://doi.org/10.2113/gsjfr.10.2.89
-
Amorphous calcium carbonate transforms into calcite during sea urchin larval spicule growthProceedings of the Royal Society of London. Series B 264:461–465.https://doi.org/10.1098/rspb.1997.0066
-
Impact of biomineralization processes on the Mg content of foraminiferal shells: A biological perspectiveGeochemistry, Geophysics, Geosystems 7:2005GC001015.https://doi.org/10.1029/2005GC001015
-
Biomineralisation bei milioliden Foraminiferen und die Matritzen-HypotheseDie Naturwissenschaften 63:196–197.https://doi.org/10.1007/BF00624226
-
BookCalcification in the coccolithophorids Emiliania huxleyi and Pleurochrysis carterae II. biochemical aspectsIn: Leadbeater BSC, editors. Biomineralization in Lower Plants and Animals. Clarendon Press. pp. 205–217.
-
Soluble adenylyl cyclase coordinates intracellular pH homeostasis and biomineralization in calcifying cells of a marine animalAmerican Journal of Physiology. Cell Physiology 324:C777–C786.https://doi.org/10.1152/ajpcell.00524.2022
-
Intracellular pH distribution in foraminifera determined by the fluorescent probe HPTSLimnology and Oceanography 6:610–618.https://doi.org/10.4319/lom.2008.6.610
-
500 million years of foraminiferal calcificationEarth-Science Reviews 243:104484.https://doi.org/10.1016/j.earscirev.2023.104484
-
Micro- and nanostructures of calcareous foraminiferal tests: insight from representatives of miliolida, rotaliida and lagenidaJournal of Foraminiferal Research 48:142–155.https://doi.org/10.2113/gsjfr.48.2.142
-
Chamber arrangement versus wall structure in the high-rank phylogenetic classification of ForaminiferaActa Palaeontologica Polonica 64:1–18.https://doi.org/10.4202/app.00564.2018
-
BookSymbiont-bearing foraminiferaIn: Hallock P, editors. Modern Foraminifera. Springer. pp. 123–139.https://doi.org/10.1007/0-306-48104-9_8
-
BookCalcification and chamber formation in foraminifera-A brief overviewIn: Leadbeater BC, Riding R, editors. Biomineralization in Lower Plants and Animals. The Systematics Association. Clarendon PressEditors. pp. 237–249.
-
Functional shell geometry of symbiont-bearing benthic ForaminiferaGalaxea, Journal of Coral Reef Studies 11:81–89.https://doi.org/10.3755/galaxea.11.81
-
Ion pathways in biomineralization: perspectives on uptake, transport, and deposition of calcium, carbonate, and phosphateJournal of the American Chemical Society 143:21100–21112.https://doi.org/10.1021/jacs.1c09174
-
Observations on Iridia diaphana, a Marine ForaminiferJournal of Protozoology 16:599–611.https://doi.org/10.1111/j.1550-7408.1969.tb02320.x
-
Controlling mineral morphologies and structures in biological and synthetic systemsChemical Reviews 108:4332–4432.https://doi.org/10.1021/cr8002856
-
New insight into the systematics and evolution of the foraminiferaMicropaleontology 59:493–527.
-
ConferenceUltrafine structure observation and pH imaging of site of calcification in Sorites orbiculusInternational Symposium on Foraminifera, Peruggia, FORAMS 2023, Grzybowski Foundation Special Publication no.27. pp. 1–194.https://doi.org/10.5194/egusphere-egu24-14624
-
Ultrastructure of the test wall in modern porcelaneous foraminifera: implications for the classification of the miliolidaJournal of Foraminiferal Research 47:136–174.https://doi.org/10.2113/gsjfr.47.2.136
-
New supraordinal classification of Foraminifera: Molecules meet morphologyMarine Micropaleontology 100:1–10.https://doi.org/10.1016/j.marmicro.2013.04.002
-
Evolutionary significance of the microbial assemblages of large benthic ForaminiferaBiological Reviews of the Cambridge Philosophical Society 94:828–848.https://doi.org/10.1111/brv.12482
-
Taxon-rich transcriptomics supports higher-level phylogeny and major evolutionary trends in ForaminiferaMolecular Phylogenetics and Evolution 174:107546.https://doi.org/10.1016/j.ympev.2022.107546
-
Mesocrystals: structural and morphogenetic aspectsChemical Society Reviews 45:5821–5833.https://doi.org/10.1039/c6cs00208k
-
Proton pumping accompanies calcification in foraminiferaNature Communications 8:14145.https://doi.org/10.1038/ncomms14145
-
Invasive Japanese foraminifera in a south-west Australian estuaryMarine and Freshwater Research 73:328–342.https://doi.org/10.1071/MF21254
-
Foraminiferal organic linings: functional and phylogenetic challengesEarth-Science Reviews 220:103726.https://doi.org/10.1016/j.earscirev.2021.103726
-
Biologically formed amorphous calcium carbonateConnective Tissue Research 44:214–218.https://doi.org/10.1080/713713619
-
Crystallization pathways in biomineralizationAnnual Review of Materials Research 41:21–40.https://doi.org/10.1146/annurev-matsci-062910-095803
-
Mollusc larval shell formation: amorphous calcium carbonate is a precursor phase for aragoniteThe Journal of Experimental Zoology 293:478–491.https://doi.org/10.1002/jez.90004
-
Chamber formation in archaias angulatusThe Journal of Foraminiferal Research 29:69–74.https://doi.org/10.2113/gsjfr.29.1.69
Article and author information
Author details
Funding
Alexander von Humboldt-Stiftung
- Zofia Dubicka
Polish National Science Center (UMO-2018/29/B/ST10/01811)
- Jarosław Tyszka
- Zofia Dubicka
The funders had no role in study design, data collection and interpretation, or the decision to submit the work for publication.
Acknowledgements
This work was supported by the Alexander von Humboldt Foundation Research Fellowship for experienced researchers to ZD and the Polish National Science Center (UMO-2018/29/B/ST10/01811) to JT and ZD, a grant coordinated by Grzegorz Racki, University of Silesia. We kindly thank Oscar Branson for his comments on an earlier version of the manuscript and the suggested improvements. We sincerely appreciate the valuable feedback and constructive criticism provided by the anonymous reviewers.
Version history
- Sent for peer review:
- Preprint posted:
- Reviewed Preprint version 1:
- Reviewed Preprint version 2:
- Version of Record published:
Cite all versions
You can cite all versions using the DOI https://doi.org/10.7554/eLife.91568. This DOI represents all versions, and will always resolve to the latest one.
Copyright
© 2024, Dubicka et al.
This article is distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use and redistribution provided that the original author and source are credited.
Metrics
-
- 511
- views
-
- 91
- downloads
-
- 0
- citations
Views, downloads and citations are aggregated across all versions of this paper published by eLife.
Download links
Downloads (link to download the article as PDF)
Open citations (links to open the citations from this article in various online reference manager services)
Cite this article (links to download the citations from this article in formats compatible with various reference manager tools)
Further reading
-
- Evolutionary Biology
The ovules or seeds (fertilized ovules) with wings are widespread and especially important for wind dispersal. However, the earliest ovules in the Famennian of the Late Devonian are rarely known about the dispersal syndrome and usually surrounded by a cupule. From Xinhang, Anhui, China, we now report a new taxon of Famennian ovules, Alasemenia tria gen. et sp. nov. Each ovule of this taxon possesses three integumentary wings evidently extending outwards, folding inwards along abaxial side and enclosing most part of nucellus. The ovule is borne terminally on smooth dichotomous branches and lacks a cupule. Alasemenia suggests that the integuments of the earliest ovules without a cupule evolved functions in probable photosynthetic nutrition and wind dispersal. It indicates that the seed wing originated earlier than other wind dispersal mechanisms such as seed plume and pappus, and that three- or four-winged seeds were followed by seeds with less wings. Mathematical analysis shows that three-winged seeds are more adapted to wind dispersal than seeds with one, two or four wings under the same condition.
-
- Evolutionary Biology
The Xerces Blue (Glaucopsyche xerces) is considered to be the first butterfly to become extinct in historical times. It was notable for its chalky lavender wings with conspicuous white spots on the ventral wings. The last individuals were collected in their restricted habitat, in the dunes near the Presidio military base in San Francisco, in 1941. We sequenced the genomes of four 80- to 100-year-old Xerces Blue, and seven historical and one modern specimens of its closest relative, the Silvery Blue (Glaucopsyche lygdamus). We compared these to a novel annotated genome of the Green-Underside Blue (Glaucopsyche alexis). Phylogenetic relationships inferred from complete mitochondrial genomes indicate that Xerces Blue was a distinct species that diverged from the Silvery Blue lineage at least 850,000 years ago. Using nuclear genomes, both species experienced population growth during the Eemian interglacial period, but the Xerces Blue decreased to a very low effective population size subsequently, a trend opposite to that observed in the Silvery Blue. Runs of homozygosity and deleterious load in the former were significantly greater than in the later, suggesting a higher incidence of inbreeding. These signals of population decline observed in Xerces Blue could be used to identify and monitor other insects threatened by human activities, whose extinction patterns are still not well known.