Daisy-chain gene drives for the alteration of local populations

If they are able to spread in wild populations, CRISPR-based gene-drive elements would provide new ways to address ecological problems by altering the traits of wild organisms, but the potential for uncontrolled spread tremendously complicates ethical development and use. Here, we detail a self-exhausting form of CRISPR-based drive system comprising genetic elements arranged in a daisy chain such that each drives the next. “Daisy-drive” systems can locally duplicate any effect achievable by using an equivalent self-propagating drive system, but their capacity to spread is limited by the successive loss of nondriving elements from one end of the chain. Releasing daisy-drive organisms constituting a small fraction of the local wild population can drive a useful genetic element nearly to local fixation for a wide range of fitness parameters without self-propagating spread. We additionally report numerous highly active guide RNA sequences sharing minimal homology that may enable evolutionarily stable daisy drive as well as self-propagating CRISPR-based gene drive. Especially when combined with threshold dependence, daisy drives could simplify decision-making and promote ethical use by enabling local communities to decide whether, when, and how to alter local ecosystems.

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Daisy-chain gene drives for the alteration of local populations

10.1101/057307 ◽

2016 ◽

Cited By ~ 30

Author(s):

Charleston Noble ◽

John Min ◽

Jason Olejarz ◽

Joanna Buchthal ◽

Alejandro Chavez ◽

...

Keyword(s):

Local Level ◽

Field Trials ◽

Local Communities ◽

Chain Gene ◽

Gene Drive ◽

Guide Rna ◽

Local Populations ◽

Wide Range ◽

Global Spread ◽

Drive Systems

AbstractRNA-guided gene drive elements could address many ecological problems by altering the traits of wild organisms, but the likelihood of global spread tremendously complicates ethical development and use. Here we detail a localized form of CRISPR-based gene drive composed of genetic elements arranged in a daisy-chain such that each element drives the next. “Daisy drive” systems can duplicate any effect achievable using an equivalent global drive system, but their capacity to spread is limited by the successive loss of non-driving elements from the base of the chain. Releasing daisy drive organisms constituting a small fraction of the local wild population can drive a useful genetic element to local fixation for a wide range of fitness parameters without resulting in global spread. We additionally report numerous highly active guide RNA sequences sharing minimal homology that may enable evolutionary stable daisy drive as well as global CRISPR-based gene drive. Daisy drives could simplify decision-making and promote ethical use by enabling local communities to decide whether, when, and how to alter local ecosystems.Author’s Summary‘Global’ gene drive systems based on CRISPR are likely to spread to every population of the target species, hampering safe and ethical use. ‘Daisy drive’ systems offer a way to alter the traits of only local populations in a temporary manner. Because they can exactly duplicate the activity of any global CRISPR-based drive at a local level, daisy drives may enable safe field trials and empower local communities to make decisions concerning their own shared environments.For more details and an animation intended for a general audience, see the summary at Sculpting Evolution.

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Gene Drives Across Engineered Fitness Valleys: Modeling a Design to Prevent Drive Spillover

10.1101/2020.10.29.360404 ◽

2020 ◽

Author(s):

Frederik J.H. de Haas ◽

Sarah P. Otto

Keyword(s):

Local Population ◽

Target Population ◽

Drive System ◽

High Threshold ◽

Gene Drive ◽

Time Model ◽

Population Replacement ◽

Low Threshold ◽

Drive Systems ◽

Gene Drives

1AbstractEngineered gene drive techniques for population replacement and/or suppression have potential for tackling complex challenges, including reducing the spread of diseases and invasive species. Unfortunately, the self-propelled behavior of drives can lead to the spread of transgenic elements beyond the target population, which is concerning. Gene drive systems with a low threshold frequency for invasion, such as homing-based gene drive systems, require initially few transgenic individuals to spread and are therefore easy to implement. However their ease of spread presents a double-edged sword; their low threshold makes these drives much more susceptible to spread outside of the target population (spillover). We model a proposed drive system that transitions in time from a low threshold drive system (homing-based gene drive) to a high threshold drive system (underdominance) using daisy chain technology. This combination leads to a spatially restricted drive strategy, while maintaining an attainable release threshold. We develop and analyze a discrete-time model as proof of concept and find that this technique effectively generates stable local population suppression, while preventing the spread of transgenic elements beyond the target population under biologically realistic parameters.

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Daisyfield gene drive systems harness repeated genomic elements as a generational clock to limit spread

10.1101/104877 ◽

2017 ◽

Cited By ~ 8

Author(s):

John Min ◽

Charleston Noble ◽

Devora Najjar ◽

Kevin M. Esvelt

Keyword(s):

Single Copy ◽

Drive System ◽

Gene Drive ◽

Wild Type ◽

Wild Populations ◽

Guide Rna ◽

Guide Rnas ◽

Multiple Copies ◽

Rna Elements ◽

Drive Systems

AbstractMethods of altering wild populations are most useful when inherently limited to local geographic areas. Here we describe a novel form of gene drive based on the introduction of multiple copies of an engineered ‘daisy’ sequence into repeated elements of the genome. Each introduced copy encodes guide RNAs that target one or more engineered loci carrying the CRISPR nuclease gene and the desired traits. When organisms encoding a drive system are released into the environment, each generation of mating with wild-type organisms will reduce the average number of the guide RNA elements per ‘daisyfield’ organism by half, serving as a generational clock. The loci encoding the nuclease and payload will exhibit drive only as long as a single copy remains, placing an inherent limit on the extent of spread.

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Genetic conversion of a split-drive into a full-drive element

10.1101/2021.12.05.471291 ◽

2021 ◽

Author(s):

Gerard Terradas ◽

Jared B. Bennett ◽

Zhiqian Li ◽

John M. Marshall ◽

Ethan Bier

Keyword(s):

Gene Drive ◽

Fitness Costs ◽

Experimental Proof ◽

Guide Rna ◽

Split Gene ◽

Core Components ◽

Beneficial Traits ◽

Drive Systems ◽

Genetic Conversion ◽

Gene Drives

AbstractGene-drive systems offer an important new avenue for spreading beneficial traits into wild populations. Their core components, Cas9 and guide RNA (gRNA), can either be linked within a single cassette (full gene drive, fGD) or provided in two separate elements (split gene drive, sGD) wherein the gRNA-bearing element drives in the presence of an independent static source of Cas9. We previously designed a system engineered to turn split into full gene drives. Here, we provide experimental proof-of-principle for such a convertible system inserted at the spo11 locus, which is recoded to restore gene function. In multigenerational cage studies, the reconstituted spo11 fGD cassette initially drives with slower kinetics than the unlinked sGD element (using the same Mendelian vasa-Cas9 source), but eventually reaches a similar level of final introgression. Different kinetic behaviors may result from transient fitness costs associated with individuals co-inheriting Cas9 and gRNA transgenes during the drive process.

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Design and analysis of CRISPR-based underdominance toxin-antidote gene drives

10.1101/861435 ◽

2019 ◽

Cited By ~ 7

Author(s):

Jackson Champer ◽

Samuel E. Champer ◽

Isabel Kim ◽

Andrew G. Clark ◽

Philipp W. Messer

Keyword(s):

Critical Frequency ◽

Essential Gene ◽

Geographic Location ◽

Early Embryo ◽

Gene Drive ◽

Wide Range ◽

Vector Borne ◽

Drive Systems ◽

Invasion Threshold ◽

Gene Drives

ABSTRACTCRISPR gene drive systems offer a mechanism for transmitting a desirable transgene throughout a population for purposes ranging from vector-borne disease control to invasive species suppression. In this simulation study, we assess the performance of several CRISPR-based underdominance gene drive constructs employing toxin-antidote principles. These drives disrupt the wild-type version of an essential gene using a CRISPR nuclease (the toxin) while simultaneously carrying a recoded version of the gene (the antidote). Drives of this nature allow for releases that could be potentially confined to a desired geographic location. This is because such drives have a nonzero invasion threshold frequency, referring to the critical frequency required for the drive to spread through the population. We model drives which target essential genes that are either haplosufficient or haplolethal, using nuclease promoters with expression restricted to the germline, promoters that additionally result in cleavage activity in the early embryo from maternal deposition, and promoters that have ubiquitous somatic expression. We also study several possible drive architectures, considering both “same-site” and “distant-site” systems, as well as several reciprocally targeting drives. Together, these drive variants provide a wide range of invasion threshold frequencies and options for both population modification and suppression. Our results suggest that CRISPR toxin-antidote underdominance drive systems could allow for the design of highly flexible and potentially confinable gene drive strategies.

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Invasion and migration of spatially self-limiting gene drives: a comparative analysis

10.1101/159855 ◽

2017 ◽

Cited By ~ 2

Author(s):

Sumit Dhole ◽

Michael R. Vella ◽

Alun L. Loyd ◽

Fred Gould

Keyword(s):

Target Population ◽

Gene Drive ◽

Fitness Costs ◽

Invasion And Migration ◽

Migration Rates ◽

Chain System ◽

Drive Systems ◽

And Migration ◽

The One ◽

Gene Drives

AbstractRecent advances in research on gene drives have produced genetic constructs that could theoretically spread a desired gene (payload) into all populations of a species, with a single release in one place. This attribute has advantages, but also comes with risks and ethical concerns. There has been a call for research on gene drive systems that are spatially and/or temporally self-limiting. Here we use a population genetics model to compare the expected characteristics of three spatially self-limiting gene drive systems: one-locus underdominance, two-locus underdominance, and daisy-chain drives. We find large differences between these gene drives in the minimum release size required for successfully driving a payload into a population. The daisy-chain system is the most efficient, requiring the smallest release, followed by the two-locus underdominance system, and then the one-locus underdominance system. However, when the target population exchanges migrants with a non-target population, the gene drives requiring smaller releases suffer from higher risks of unintended spread. For payloads that incur relatively low fitness costs (up to 30%), a simple daisy-chain drive is practically incapable of remaining localized, even with migration rates as low as 0.5% per generation. The two-locus underdominance system can achieve localized spread under a broader range of migration rates and of payload fitness costs, while the one-locus underdominance system largely remains localized. We also find differences in the extent of population alteration and in the permanence of the alteration achieved by the three gene drives. The two-locus underdominance system does not always spread the payload to fixation, even after successful drive, while the daisy-chain system can, for a small set of parameter values, achieve a temporally-limited spread of the payload. These differences could affect the suitability of each gene drive for specific applications.Note:This manuscript has been accepted for publication in the journal Evolutionary Applications and is pending publication. We suggest that any reference to or quotation of this article should be made with this recognition.

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Evolutionary dynamics of CRISPR gene drives

10.1101/057281 ◽

2016 ◽

Cited By ~ 10

Author(s):

Charleston Noble ◽

Jason Olejarz ◽

Kevin M. Esvelt ◽

George M. Church ◽

Martin A. Nowak

Keyword(s):

Evolutionary Dynamics ◽

Evolutionary Stability ◽

Clear Understanding ◽

Gene Drive ◽

Host Organism ◽

Wild Populations ◽

Selfish Genetic Elements ◽

Real World Applications ◽

Drive Systems ◽

Gene Drives

AbstractThe alteration of wild populations has been discussed as a solution to a number of humanity’s most pressing ecological and public health concerns. Enabled by the recent revolution in genome editing, CRISPR gene drives, selfish genetic elements which can spread through populations even if they confer no advantage to their host organism, are rapidly emerging as the most promising approach. But before real-world applications are considered, it is imperative to develop a clear understanding of the outcomes of drive release in nature. Toward this aim, we mathematically study the evolutionary dynamics of CRISPR gene drives. We demonstrate that the emergence of drive-resistant alleles presents a major challenge to previously reported constructs, and we show that an alternative design which selects against resistant alleles greatly improves evolutionary stability. We discuss all results in the context of CRISPR technology and provide insights which inform the engineering of practical gene drive systems.

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Dodging silver bullets: good CRISPR gene-drive design is critical for eradicating exotic vertebrates

Proceedings of The Royal Society B Biological Sciences ◽

10.1098/rspb.2017.0799 ◽

2017 ◽

Vol 284 (1860) ◽

pp. 20170799 ◽

Cited By ~ 58

Author(s):

Thomas A. A. Prowse ◽

Phillip Cassey ◽

Joshua V. Ross ◽

Chandran Pfitzner ◽

Talia A. Wittmann ◽

...

Keyword(s):

Female Sterility ◽

Gene Drive ◽

End Joining ◽

Guide Rna ◽

Deleterious Alleles ◽

Precise Knowledge ◽

Animal Populations ◽

Individual Based Models ◽

Non Homologous End Joining ◽

Gene Drives

Self-replicating gene drives that can spread deleterious alleles through animal populations have been promoted as a much needed but controversial ‘silver bullet’ for controlling invasive alien species. Homing-based drives comprise an endonuclease and a guide RNA (gRNA) that are replicated during meiosis via homologous recombination. However, their efficacy for controlling wild populations is threatened by inherent polymorphic resistance and the creation of resistance alleles via non-homologous end-joining (NHEJ)-mediated DNA repair. We used stochastic individual-based models to identify realistic gene-drive strategies capable of eradicating vertebrate pest populations (mice, rats and rabbits) on islands. One popular strategy, a sex-reversing drive that converts heterozygous females into sterile males, failed to spread and required the ongoing deployment of gene-drive carriers to achieve eradication. Under alternative strategies, multiplexed gRNAs could overcome inherent polymorphic resistance and were required for eradication success even when the probability of NHEJ was low. Strategies causing homozygotic embryonic non-viability or homozygotic female sterility produced high probabilities of eradication and were robust to NHEJ-mediated deletion of the DNA sequence between multiplexed endonuclease recognition sites. The latter two strategies also purged the gene drive when eradication failed, therefore posing lower long-term risk should animals escape beyond target islands. Multiplexing gRNAs will be necessary if this technology is to be useful for insular extirpation attempts; however, precise knowledge of homing rates will be required to design low-risk gene drives with high probabilities of eradication success.

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Molecular safeguarding of CRISPR gene drive experiments

eLife ◽

10.7554/elife.41439 ◽

2019 ◽

Vol 8 ◽

Cited By ~ 39

Author(s):

Jackson Champer ◽

Joan Chung ◽

Yoo Lim Lee ◽

Chen Liu ◽

Emily Yang ◽

...

Keyword(s):

Drosophila Melanogaster ◽

Natural Population ◽

Early Embryo ◽

Drive System ◽

Target Site ◽

Gene Drive ◽

Gene Drives ◽

Synthetic Target

CRISPR-based homing gene drives have sparked both enthusiasm and deep concerns due to their potential for genetically altering entire species. This raises the question about our ability to prevent the unintended spread of such drives from the laboratory into a natural population. Here, we experimentally demonstrate the suitability of synthetic target site drives as well as split drives as flexible safeguarding strategies for gene drive experiments by showing that their performance closely resembles that of standard homing drives in Drosophila melanogaster. Using our split drive system, we further find that maternal deposition of both Cas9 and gRNA is required to form resistance alleles in the early embryo and that maternally-deposited Cas9 alone can power germline drive conversion in individuals that lack a genomic source of Cas9.

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Small-molecule control of super-Mendelian inheritance in gene drives

10.1101/665620 ◽

2019 ◽

Cited By ~ 3

Author(s):

Víctor López Del Amo ◽

Brittany S. Leger ◽

Kurt J. Cox ◽

Shubhroz Gill ◽

Alena L. Bishop ◽

...

Keyword(s):

Small Molecule ◽

Chemical Control ◽

Control Strategies ◽

Mendelian Inheritance ◽

Drive System ◽

Gene Drive ◽

Crop Pests ◽

Vector Borne Diseases ◽

Vector Borne ◽

Gene Drives

ABSTRACTBy surpassing the 50% inheritance limit of Mendel’s law of independent assortment, CRISPR-based gene drives have the potential to fight vector-borne diseases or suppress crop pests. However, contemporary gene drives could spread unchecked, posing safety concerns that limit their use in both laboratory and field settings. Current technologies also lack chemical control strategies, which could be applied in the field for dose, spatial and temporal control of gene drives. We describe in Drosophila the first gene-drive system controlled by an engineered Cas9 and a synthetic, orally-available small molecule.Graphical Abstract

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