Rise of the Other Kind(s): Part II

Maliha Tanjum Chowdhury
Freshman
School of Life Sciences
Independent University, Bangladesh 

July 6th, 2017 

This is the second in a three-part series that will broadly introduce and describe the study of evolution using microbes as model systems, and specifically focus on a recent study on speciation.

Practically, the fastest shift from one type of organism to another that can be observed in a laboratory is that of asexual microbes, e.g. bacteria and viruses. It is needless to say that for uncomplicated, single-celled chaps like viruses, bacteria and the like, rapid transition through numerous generations in a couple of hours or less is a walk in the park. Recall that any sort of genetic variation is simply the outcome of random, independent mutations in nucleotide or gene sequences. The accumulation of major changes which can possibly be observed between consecutive generations is far more evident in the case of microbes, as the hereditary fate of a given microbe is often entirely wielded by a single strand of DNA or RNA. We can select for some of these changes by providing different selection pressures.

However, speciation, based on our textbook definition, requires the incidence of sexual reproduction for organisms to diverge into distinct species (for them to no longer be reproductively compatible). Therefore, it is harder to define species when it comes to asexual microbes. 

In a recent study exploring sympatric and allopatric speciation, bacteriophage (viruses that infect bacteria) lambda was chosen as the model system to study the processes, as it not only divides rapidly asexually, but also has an exceptional ability to recombine with phages that coinfect the same host, thereby creating progeny and exchanging genes sexually. This allowed the conclusion of the study to be at least partially relevant to sexually reproducing species. Now, even though the rates and mechanisms of speciation may seem to vary for viruses and multicellular organisms, some features are comparable. For instance, reproductive isolation and incompatibility, which are concepts we learnt about earlier, mean much the same for viruses. In this specific case, reproductive incompatibility refers to the inability to recombine with other viruses whose nucleotide composition has evolved to differ considerably. Hence, all things considered, this was a clever model to work with.

We’re now going to delve deep into the experiment itself, so hold on to your seats, because it’s going to get much more science-y from here onwards. The researchers basically tried to observe the two kinds of speciation, allopatric (due to geographical separation) and sympatric (within the same environment), respectively, in the bacteriophage populations. The lab-generated bacteriophage lambda strain EvoC was the focus of the study. Bacteriophages begin their replication cycles by binding to receptor proteins on the host cell, and injecting their genomes into the cell. Individual bacteriophages tend to be very specific to the type and structure of the receptor proteins they can bind to. This virus, however, was a “generalist”- a bacteriophage with the ability to bind to both the OmpF and LamB receptor-proteins on the bacterial surface of Escherichia Coli.  

For this study, two different hosts were utilized: an E. coli strain carrying the OmpF receptor, and an E. coli strain carrying the LamB receptor. A broad summary of the experimental results is as follows: the bacteriophages, when supplied with just one of the two hosts, specialized in binding to the available receptor on that host while steadily losing the ability to bind to the other (allopatry).  More excitingly, when propagated on equal amounts of both hosts (and therefore in the presence of both receptors) together, the bacteriophages still divided into two distinct lineages with different host preferences (sympatry). In the light of these findings, the results shine through as compelling evidence that for the advent of distinct species, both allopatry and sympatry could play significant roles.

I personally feel that this article would remain terribly incomplete without including a walk-through of the methods used. So, here they are as follows:

  1. Twelve bacteriophage (EvoC) populations, initially exactly the same, were grown with either one or other type of host, that is, six populations were grown in OmpF-expressing bacteria and the other six were grown in the LamB-expressing ones.
  2. The bacteriophage populations were systematically passaged through the host populations for 35 cycles of dilution (the experiment took roughly a month in real world time).
  3. In 8-hour intervals, bacteriophages were collected and stored.
  4.  A fresh cycle of viral reproduction was kicked off by the transfer of 1% of the phage into a brand new population of host bacteria the next day.
  5. Six other bacteriophage (EvoC) populations, initially exactly the same, were exposed to a culture of both types of host populations present in equal amounts, i.e. both OmpF and Lamb-carrying bacteria.
  6. Steps 2-4 were conducted for these as well.

Step 1 is the allopatric set-up, as the isolated flasks containing only kind of host receptor represent geographical separation and different conditions from viruses growing only with the other type of receptor. Step 5 describes the sympatric experimental set-up, as viruses are allowed to switch between both available hosts and this may allow recombination between viruses that co-infect a given bacteria at some point. Lastly, to ensure a higher chance of co-infection – and thus, recombination between viruses – a high virus to bacteria ratio was maintained in all experimental units.


 A typical plaque assay. ASM

The results, as I passingly mentioned above, were beyond satisfactory. The scientists made their primary inferences based on observing clear regions, or “holes”, in lawns of bacterial colonies grown on standard agar plates.  This experimental method is known as the plaque assay – where the term “plaque” refers to the “holes” caused by viral growth. The plaques represent the ability of the bacteriophage to bind to the bacterial receptor. If there are no plaques, there has been no binding or infection.

Considerable significant receptor specialization evolved in all 12 bacteriophage populations which were grown on single bacterial hosts, and this conclusion was drawn on observation that bacteriophages that produced plaques on OmpF-expressing bacteria failed to do so on LamB-expressing ones, and vice versa. Again, more surprisingly, this was seen to be true for bacteriophages that were grown with both kinds of hosts together.

Therefore, even when both receptors were available, bacteriophages tended to become specialized for one kind of host. How and why might that be the case? What do these results really say about speciation? Find out the in the concluding part of this series next week. 

To be continued


Maliha is a weirdo who somehow believes she's from a different planet. But she likes Earth just fine, and is fascinated by the science and beauty of life and has made it her purpose to explore it. Besides this, her most burning desires include becoming a synthetic biologist/ genetic engineer and running away with a heavy metal band.










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